CA2371975A1 - Liquid measuring device and method of using - Google Patents
Liquid measuring device and method of using Download PDFInfo
- Publication number
- CA2371975A1 CA2371975A1 CA002371975A CA2371975A CA2371975A1 CA 2371975 A1 CA2371975 A1 CA 2371975A1 CA 002371975 A CA002371975 A CA 002371975A CA 2371975 A CA2371975 A CA 2371975A CA 2371975 A1 CA2371975 A1 CA 2371975A1
- Authority
- CA
- Canada
- Prior art keywords
- liquid
- measuring device
- mmole
- barrier
- barrel
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Abandoned
Links
Classifications
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01F—MEASURING VOLUME, VOLUME FLOW, MASS FLOW OR LIQUID LEVEL; METERING BY VOLUME
- G01F22/00—Methods or apparatus for measuring volume of fluids or fluent solid material, not otherwise provided for
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N1/00—Sampling; Preparing specimens for investigation
- G01N1/02—Devices for withdrawing samples
- G01N1/10—Devices for withdrawing samples in the liquid or fluent state
- G01N1/14—Suction devices, e.g. pumps; Ejector devices
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L3/00—Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
- B01L3/02—Burettes; Pipettes
- B01L3/021—Pipettes, i.e. with only one conduit for withdrawing and redistributing liquids
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L3/00—Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
- B01L3/02—Burettes; Pipettes
- B01L3/021—Pipettes, i.e. with only one conduit for withdrawing and redistributing liquids
- B01L3/0217—Pipettes, i.e. with only one conduit for withdrawing and redistributing liquids of the plunger pump type
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01F—MEASURING VOLUME, VOLUME FLOW, MASS FLOW OR LIQUID LEVEL; METERING BY VOLUME
- G01F19/00—Calibrated capacity measures for fluids or fluent solid material, e.g. measuring cups
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N35/00—Automatic analysis not limited to methods or materials provided for in any single one of groups G01N1/00 - G01N33/00; Handling materials therefor
- G01N35/10—Devices for transferring samples or any liquids to, in, or from, the analysis apparatus, e.g. suction devices, injection devices
- G01N35/1095—Devices for transferring samples or any liquids to, in, or from, the analysis apparatus, e.g. suction devices, injection devices for supplying the samples to flow-through analysers
- G01N35/1097—Devices for transferring samples or any liquids to, in, or from, the analysis apparatus, e.g. suction devices, injection devices for supplying the samples to flow-through analysers characterised by the valves
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2200/00—Solutions for specific problems relating to chemical or physical laboratory apparatus
- B01L2200/06—Fluid handling related problems
- B01L2200/0605—Metering of fluids
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2300/00—Additional constructional details
- B01L2300/06—Auxiliary integrated devices, integrated components
- B01L2300/0681—Filter
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2400/00—Moving or stopping fluids
- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0475—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure
- B01L2400/0478—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure pistons
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2400/00—Moving or stopping fluids
- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0475—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure
- B01L2400/0487—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure fluid pressure, pneumatics
- B01L2400/049—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure fluid pressure, pneumatics vacuum
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L3/00—Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
- B01L3/02—Burettes; Pipettes
- B01L3/0203—Burettes, i.e. for withdrawing and redistributing liquids through different conduits
- B01L3/0206—Burettes, i.e. for withdrawing and redistributing liquids through different conduits of the plunger pump type
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N35/00—Automatic analysis not limited to methods or materials provided for in any single one of groups G01N1/00 - G01N33/00; Handling materials therefor
- G01N35/10—Devices for transferring samples or any liquids to, in, or from, the analysis apparatus, e.g. suction devices, injection devices
- G01N35/1009—Characterised by arrangements for controlling the aspiration or dispense of liquids
- G01N35/1016—Control of the volume dispensed or introduced
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10T—TECHNICAL SUBJECTS COVERED BY FORMER US CLASSIFICATION
- Y10T436/00—Chemistry: analytical and immunological testing
- Y10T436/20—Oxygen containing
- Y10T436/200833—Carbonyl, ether, aldehyde or ketone containing
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10T—TECHNICAL SUBJECTS COVERED BY FORMER US CLASSIFICATION
- Y10T436/00—Chemistry: analytical and immunological testing
- Y10T436/25—Chemistry: analytical and immunological testing including sample preparation
- Y10T436/25375—Liberation or purification of sample or separation of material from a sample [e.g., filtering, centrifuging, etc.]
- Y10T436/255—Liberation or purification of sample or separation of material from a sample [e.g., filtering, centrifuging, etc.] including use of a solid sorbent, semipermeable membrane, or liquid extraction
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10T—TECHNICAL SUBJECTS COVERED BY FORMER US CLASSIFICATION
- Y10T436/00—Chemistry: analytical and immunological testing
- Y10T436/25—Chemistry: analytical and immunological testing including sample preparation
- Y10T436/2575—Volumetric liquid transfer
Abstract
A liquid measuring device is described for carrying out the assay using a gas or vapor permeable but liquid impermeable membrane barrier to control the volume of liquid to be measured or transferred. The membrane may be used in any instance where a fixed volume of liquid needs to be measured.
Description
LIQUID MEASURING DEVICE AND METHOD OF USING
Background of the Invention S Field of the Invention The Held of the invention relates to an apparatus and a method for using the apparatus for the measurement and/or transfer of a fixed volume of liquid sample.
Description of the Related Art General methods to determine a-phthalaldehyde (OPA) or glutaraldehyde concentrations are mainly instrumental measurements that could be classified into chromatographic measurement (chromatographic, HPLC analysis) or non-chromatographic measurement (direct spectroscopic assay). For HPLC analysis, OPA
or glutaraldehyde are measured by both a derivative method or a non-derivative method. The most common derivative method is to convert OPA or glutaraldehyde to 2,4-dinotrophenylhydrazones by reacting OPA with 2,4-dinitrophenylhydrazine.
Since the UV absorption is greatly enhanced, this method is valuable for low level OPA or glutaraldehyde measurements especially in environmental analysis. For measurements of high concentrations of OPA or glutaraldehyde, such as the OPA or glutaraldehyde disinfectants, OPA or glutaraldehyde could be measured directly without making derivatives first. OPA or glutaraldehyde may be analyzed easily with GC
analysis. For non-chromatographic analysis, OPA or glutaraldehyde could be measured directly with spectrophotometric methods. However, one drawback to this method is that there must be no interference at the specific wavelength used. For example, OPA or glutaraldehyde could be oxidized slowly by air and the carboxylic acid formed may interfere in such assays.
All three instrumental methods involve the preparation of samples and use of an instrument. They are all time-consuming and too expensive or too complicated for hospital end users. Therefore, Albert Browne and 3M have developed a simple strip procedure for a Pass/Fail test. In such a test, the strip was dipped into either OPA or glutaraldehyde solutions for a certain amount of time. After a predetermined time, the strip color was compared with some standard colors. Their strip chemistry principles were not released. The problems with this method are consistency and accuracy.
The strip method has the following problems ( 1 ), Good solutions (OPA or glutaraldehyde higher than "POI", the point of interest) often fail the test for different reasons. (2). The soaking time and waiting time have to be controlled carefully. Any deviation will lead to different shades of color and a false reading. (3). Moving of the strip when soaking will lead to the loss of chemical reagents to the OPA or glutaraldehyde solutions leading to false reading. (4). Individual users have different color recognition habits and often have a different opinion of the end-color. (5). The final color is dependent on many factors and is particularly sensitive to time.
The current invention provides another method without the above problems.
Although the chemistry principle could also be used for the strip approach, in a preferred embodiment it is used for the color change of a solution.
Summary of the Invention The present invention pertain to a liquid measuring device that measures a fixed volume of liquid including a first barrel having a proximal and distal end and a gas or vapor permeable but liquid impermeable barrier situated in the barrel between the proximal and distal ends, whereby the liquid can only be filled up to the barr7er. In a preferred embodiment, the volume in the barrel up to the barrier equals the fixed volume. The liquid measuring may further include a means to position the barrier to deliver a fixed volume of liquid, whereby the liquid can only be filled up to the barrier.
In a preferred embodiment, the liquid measuring device further includes a coupling device to adapt the barrier to the measuring device. In a more preferred embodiment, the coupling device includes an insert. In a most preferred embodiment, the insert is movable in the barrel. In another most preferred embodiment, the liquid measuring device further includes a holder to position and secure the insert in the liquid measuring device. In an alternate prefen-ed embodiment, the insert is moved to a desired position by means of a screw.
In a preferred embodiment, the liquid measuring device is a pipette or syringe.
In a preferred embodiment, the liquid measuring device further includes a second barrel which is in fluid communication with said first barrel by means of a valve. In a preferred embodiment, the valve is a one-way valve. In an alternate preferred embodiment, the valve has an on/off switch.
In a preferred embodiment, the liquid measuring device may further include a needle at the distal end.
In a preferred embodiment, the insert of the liquid measuring device is H-shaped in cross-sectional view. In an alternate preferred embodiment, the insert is U-shaped in cross-sectional view.
In a preferred embodiment, the first barrel of the liquid measuring device includes a valve at the distal end. In a more preferred embodiment, the valve is a one-way valve. In an alternate more preferred embodiment, the valve is an on/off valve. In a preferred embodiment, the gas or vapor permeable but liquid impermeable barrier of the liquid measuring device comprises hydrophobic material.
The present disclosure also pertains to a method of measuring a fixed volume of liquid including the steps of l ) providing a gas or vapor permeable but liquid impermeable barner in a barrel having a proximal end and a distal end;
2) inserting the distal end into a sample comprising liquid fluid;
Background of the Invention S Field of the Invention The Held of the invention relates to an apparatus and a method for using the apparatus for the measurement and/or transfer of a fixed volume of liquid sample.
Description of the Related Art General methods to determine a-phthalaldehyde (OPA) or glutaraldehyde concentrations are mainly instrumental measurements that could be classified into chromatographic measurement (chromatographic, HPLC analysis) or non-chromatographic measurement (direct spectroscopic assay). For HPLC analysis, OPA
or glutaraldehyde are measured by both a derivative method or a non-derivative method. The most common derivative method is to convert OPA or glutaraldehyde to 2,4-dinotrophenylhydrazones by reacting OPA with 2,4-dinitrophenylhydrazine.
Since the UV absorption is greatly enhanced, this method is valuable for low level OPA or glutaraldehyde measurements especially in environmental analysis. For measurements of high concentrations of OPA or glutaraldehyde, such as the OPA or glutaraldehyde disinfectants, OPA or glutaraldehyde could be measured directly without making derivatives first. OPA or glutaraldehyde may be analyzed easily with GC
analysis. For non-chromatographic analysis, OPA or glutaraldehyde could be measured directly with spectrophotometric methods. However, one drawback to this method is that there must be no interference at the specific wavelength used. For example, OPA or glutaraldehyde could be oxidized slowly by air and the carboxylic acid formed may interfere in such assays.
All three instrumental methods involve the preparation of samples and use of an instrument. They are all time-consuming and too expensive or too complicated for hospital end users. Therefore, Albert Browne and 3M have developed a simple strip procedure for a Pass/Fail test. In such a test, the strip was dipped into either OPA or glutaraldehyde solutions for a certain amount of time. After a predetermined time, the strip color was compared with some standard colors. Their strip chemistry principles were not released. The problems with this method are consistency and accuracy.
The strip method has the following problems ( 1 ), Good solutions (OPA or glutaraldehyde higher than "POI", the point of interest) often fail the test for different reasons. (2). The soaking time and waiting time have to be controlled carefully. Any deviation will lead to different shades of color and a false reading. (3). Moving of the strip when soaking will lead to the loss of chemical reagents to the OPA or glutaraldehyde solutions leading to false reading. (4). Individual users have different color recognition habits and often have a different opinion of the end-color. (5). The final color is dependent on many factors and is particularly sensitive to time.
The current invention provides another method without the above problems.
Although the chemistry principle could also be used for the strip approach, in a preferred embodiment it is used for the color change of a solution.
Summary of the Invention The present invention pertain to a liquid measuring device that measures a fixed volume of liquid including a first barrel having a proximal and distal end and a gas or vapor permeable but liquid impermeable barrier situated in the barrel between the proximal and distal ends, whereby the liquid can only be filled up to the barr7er. In a preferred embodiment, the volume in the barrel up to the barrier equals the fixed volume. The liquid measuring may further include a means to position the barrier to deliver a fixed volume of liquid, whereby the liquid can only be filled up to the barrier.
In a preferred embodiment, the liquid measuring device further includes a coupling device to adapt the barrier to the measuring device. In a more preferred embodiment, the coupling device includes an insert. In a most preferred embodiment, the insert is movable in the barrel. In another most preferred embodiment, the liquid measuring device further includes a holder to position and secure the insert in the liquid measuring device. In an alternate prefen-ed embodiment, the insert is moved to a desired position by means of a screw.
In a preferred embodiment, the liquid measuring device is a pipette or syringe.
In a preferred embodiment, the liquid measuring device further includes a second barrel which is in fluid communication with said first barrel by means of a valve. In a preferred embodiment, the valve is a one-way valve. In an alternate preferred embodiment, the valve has an on/off switch.
In a preferred embodiment, the liquid measuring device may further include a needle at the distal end.
In a preferred embodiment, the insert of the liquid measuring device is H-shaped in cross-sectional view. In an alternate preferred embodiment, the insert is U-shaped in cross-sectional view.
In a preferred embodiment, the first barrel of the liquid measuring device includes a valve at the distal end. In a more preferred embodiment, the valve is a one-way valve. In an alternate more preferred embodiment, the valve is an on/off valve. In a preferred embodiment, the gas or vapor permeable but liquid impermeable barrier of the liquid measuring device comprises hydrophobic material.
The present disclosure also pertains to a method of measuring a fixed volume of liquid including the steps of l ) providing a gas or vapor permeable but liquid impermeable barner in a barrel having a proximal end and a distal end;
2) inserting the distal end into a sample comprising liquid fluid;
3) creating a negative pressure on the proximal end; and 4) transferring the liquid tluid from the sample into the barrel, wherein the liquid fluid can only be filled up to the barrier.
In a preferred embodiment, the method further includes adjusting the position of the barrier in the barrel. In a preferued embodiment, the barrier is part of a coupling device and the method further includes adapting the coupling device to the barrel. In a more preferred embodiment, the adapting includes inserting the coupling device into ?5 the barrel.
In a preferred embodiment, the barrel further includes a valve at the distal end and the method further includes opening and/or closing the valve.
In a preferred embodiment, the method further includes pulling a plunger in the barner to create a negative pressure.
For purposes of summarizing the invention and the advantages achieved over the prior art, certain objects and advantages of the invention have been described above. Of course, it is to be understood that not necessarily all such objects or advantages may be achieved in accordance with any particular embodiment of the invention. Thus, for example, those skilled in the art will recognize that the invention may be embodied or carried out in a manner that achieves or optimizes one advantage or group of advantages as taught herein without necessarily achieving other objects or advantages as may be taught or suggested herein.
Further aspects, features and advantages of this invention will become apparent from the detailed description of the preferred embodiments which follow.
Brief Description of the Drawings These and other feature of this invention will now be described with reference to the drawings of preferred embodiments which are intended to illustrate and not to limit the invention.
Figure 1 shows the basic principles of the described assay. Reaction 1 shows the reaction of aldehyde with compound X to produce a compound with a first color.
Preferably, the first color is colorless. Reaction ? shows the reaction of aldehyde and Y
to form a compound with a second color. Preferably, reaction 2 is slower than Reaction 1. If the concentration of aldehyde is below the POI (point of interest) only compound X will react and the resulting solution will be the first color as shown in the bottom half ?0 of the figure. In the presence of a level of aldehyde that is equal to or more than the PUI, a solution with the second color or the combined color of the first color and the second color will be formed.
Figure ? shows a pipette and two variants of a syringe with a gas or vapor permeable liquid impermeable barrier.
Figure 3A shows the coupling of the gas or vapor permeable liquid impermeable barrier to the syringe or pipette. Figure 3B illustrates how inserts 4 at the top of the pipette or syringe attach the gas or vapor permeable liquid impermeable barrier to the pipette or syringe. Figure 3C illustrates a holder 5 that holds the inserts in place.
Figure 3D shows the inserts and the coupling of the gas or vapor permeable liquid impermeable barrier.
Figure 4 is an expanded view of figure 3C which shows a gas or vapor permeable liquid impermeable barner l, an insert 4, and a holder 5.
Figure 5 shows one embodiment of the invention where the position of the gas or vapor permeable liquid impermeable membrane is adjusted by means of a screw.
Figures 6A and 6B show embodiments of the liquid delivery apparatus with all chemicals in one chamber. Figure 6C shows a two chambered embodiment of the liquid delivery apparatus. The test sample may be taken into the first chamber for reaction with the first compound such as compound X in Figure 1. Then the sample is moved by means of a one-way valve or a manual ON/OFF valve 8 into the second chamber where the test sample reacts with the second compound such as compound Y
of Figure 1.
Detailed Description of the Preferred Embodiment While the described embodiment represents the preferred embodiment of the present invention, it is to be understood that modifications will occur to those skilled in the art without departing from the spirit of the invention. The scope of the invention is therefore to be determined solely by the appended claims.
Aldehydes react with amino-containing compounds like amino acids or amines to form an imine or more commonly known as a Schiff's base, which is often colored.
Taking glycine as an example:
p N
() ~ ~--()H
~H ~ O
? H=N () H ~<>ri (>H
() r ? 3 ((srecn to r3lack, changine Irom li~~hter to darker) Schiff's Base Formation between OPA and Glycine Another known aldehyde reaction is the sodium bisulfate carbonyl addition reaction.
O UH
H ~ ~ ~SO;Na + 2 NaHSO; SOjNa H
O OH
t a (Colol'Iess) Addition Reaction of Sodium Bisulfate to OPA
The sodium bisulfate addition reaction is more favorable than that of Schiff's formation since the former reaction is fast and hard to reverse. Thus, in the presence of both a compound containing an amino group such as an amino acid and a reagent such as sodium bisulfate, the aldehyde will react first with sodium bisulfate and then with the amino acid. Therefore, it is possible to design a color pass/fail reaction by controlling the amount of reagents to react with aldehydes such as formaldehyde, OPA or glutaraldehyde. The key is the amount of reagent such as sodium bisulfate which is designed to react with the aldehyde without a color being developed in the presence of I S an amino acid. Any remaining aldehyde will then react with the amino acid to develop a colored solution. This confirms the presence of a certain amount of an aldehyde such as formaldehyde, OPA or glutaraldehyde in a test solution such as a disinfectant solution. On the other hand, if no color was developed, it confirms that the formaldehyde, OPA or glutaraldehyde concentration is below an acceptable specitication. The specific concentration can be set to any point by adjusting the amounts of the chemical reagents used or by using different amounts of aldehyde (formaldehyde, OPA or glutaraldehyde) in the test solution.
Thus, a color pass/fail reaction for determination of excess aldehyde by control of reagents which react with aldehyde is described. The key is the amount of reagent ?5 such as sodium bisulfate which is designed to react with the Point of Interest (POI) level of aldehyde without a color being developed in the presence of a compound containing an amino group such as an amino acid. Any ''extra" aldehyde, exceeding the POI, will then react with the compound containing an amino group, causing a color to be developed. In a preferred embodiment, the aldehyde is either OPA or glutaraldehyde and the compound containing the amino group is an amino acid. This method is especially useful for quality control where components only needed to be examined in pre-determined ranges.
A number of reagents which are known to react quickly with aldehydes may be used in the practice of the invention. These include any chemicals which can oxidize or reduce the aldehyde group and any chemicals which can react with and alter the carbonyl functional group of the aldehyde. Examples of such reagents are disclosed in Morrison & Boyd, "Organic Chemistry", Chapter 19, Allyn and Bacon, 3"~
edition, 1973, which is herein incorporated by reference. Such reagents include, but are not limited to, Ag(NH3)~; KMnO~; K,Cr~O~; H, + Ni, Pt, or Pd; LiAIHa or NaBH.~, then H+;
Zn (Hg), conc. HCI; NH~NHZ, base; Grignard reagents; salts of cyanide and bisulfite;
ammonia derivatives such as hydroxylamine, hydrazine, phenylhydrazine, and semicarbazide; reactions with alcohols in the presence of acid; and reactions with acid or base such as the Cannizzaro reaction, the aldol condensation, and the Perkin condensation. In a preferred embodiment, the reagent which reacts with the aldehyde is a salt of either bisulfite or cyanide.
This aspect of the invention is illustrated in Figure 1. Both compounds X and Y react with the aldehyde in the figure. Preferably X reacts much faster than Y.
?0 Preferably, the reaction of X with aldehyde results in a colorless compound whereas the reaction of Y with aldehyde results in a colored compound. A point of interest is chosen and the amount of X that will react with the point of interest is determined.
When the aldehyde is mixed with X and Y, the aldehyde will react first with compound X which is kinetically and thermodynamically favored. Any excess aldehyde will then react with compound Y to form a colored solution.
Consequently, if a colored solution results, the concentration of aldehyde is above the point of interest. The determination may be made visually, with or without a color chart.
Alternatively, a spectrophotometer may be used. If the reaction between the aldehyde and compound X is not kinetically and thermodynamically favored, then compound Y
can be added after the aldehyde reacts with compound X as shown in Figure 1.
_7_ The theoretical amount of OPA: sodium bisulfate is I :2. However, it was found that less sodium bisulfate is needed to react with OPA than the theoretical amount in order to get a good color display.
Another aspect of the invention is a liquid-measuring device, such as a pipette or syringe, for carrying out the assay. This device could be used for any "faxed-volume" measurement and transfer in chemistry, biochemistry, clinical chemistry or other industries.
The apparatus may be a syringe or pipette with one or more barrels and plungers and a membrane barrier with or without a coupling device. The membrane barrier is a gas or vapor permeable and liquid impermeable barrier. In the presence of certain pressure differences between the two sides of the barrier, the gas or vapor flows through the membrane but not the liquid. Any suitable gas or vapor permeable and liquid impermeable materials can be used for this purpose. Some examples include, but are not limited to, nonwoven polyolefin, such as Tyvek~a~~a (non-woven polyethylene), or CSR (non-woven polypropylene central supply room), wrapping material and any other hydrophobic filtering materials. Optionally, the device contains an insert and a holder.
The syringe or pipette apparatus may also contain valves to control the flow of liquid.
The membrane barrier can be thermally bound to the syringe or pipet. It can also be attached to the syringe or pipet with an adhesive or connected to the syringe barrel by a coupling device. The coupling device may be connected to an insert for altering the position of the membrane barrier. The position of the membrane barrier can be adjusted by the length of the insert. The insert may be secured with a holder.
The membrane barner is a gas or vapor permeable but liquid impermeable barrier. The membrane barrier is positioned such that the liquid can only be tilled up to the barrier. The invention has several preferred embodiments.
In the first embodiment (Figure 2), a gas or vapor permeable liquid impermeable membrane 1 is fixed into the pipette 7 or syringe 6 and held in place at the desired maximum volume by means known in the art. The syringe includes a plunger 3.
The syringe can have a metal or plastic needle with or without a needle cap. In one embodiment (Figures 3A-3D), a coupling device 2 is used which is larger or smaller _g_ than the diameter of the pipette 7 or syringe 6. Two parts of the pipet or syringe with different lengths can be joined together with such a coupling device.
Coupling of the membrane barrier to the syringe or pipette is shown in Figures 3A, 3B, 3C, 3D and Figure 4. The membrane can be inserted into the syringe or pipet from the top of the pipette or syringe by an insert 4 which may be secured with a holder 5 and its position varied by any means known in the art such as by a screw (Figure 5) or a slidable adjustment (Figure 4j. Figure 3D shows an insert which has a larger diameter than the pipette or syringe. By adjusting the insert and creating a negative pressure on the upper part of the pipette or syringe, the fluid can be loaded into the syringe or pipette up to the barrier.
Figures 6A, 6B and 6C illustrate the use of the measuring device with this invention. Figures 6A and 6B show a syringe with a gas or vapor permeable liquid impermeable barrier and two chemicals. The liquid can be filled in the syringe by inserting the plastic needle into the sample solution, pulling the plunger to create a negative pressure in the syringe, and loading the liquid into the syringe. The measuring device can have a filtering material (Figure 6A) or valve (Figure 6B) to retain the chemicals in the barrel. The chemical in the syringe can be in either a liquid or solid form. The valve can be a one-way valve or a manual ON/OFF valve.
Figure 6C provides another embodiment for mixing more than one reactant successively. It has two chambers 9, 10. A fixed volume of any solution including, but not limited to an aldehyde is drawn up through a one-way valve or an ON/OFF
valve 8 into the first chamber 9 where it mixes with the first reactant, for example sodium bisulfite. After a predetermined time, the reactants flow through a second one-way valve or an ONIOFF valve 8 into a second reaction chamber 10 which might contain an amine such as lysine, for example, to complete the reaction.
Alternatively, a three-way valve can be used instead of two one-way valves.
The invention has several advantages over the prior art methods. First, the pass/fail conclusion is consistent and convenient. Preferably, there is no need to guess the color. The user's only conclusion will be "colored" or "not colored."
Second, the liquid transferring device is consistent and convenient. A fixed volume of liquid can be taken by a simple operation. Third, the solution color is easier to visualize than a test strip paper since the test strip paper itself is colored, leading to false positive results.
Fourth, the color displaying time can be adjusted by adding a base to make the reaction faster or an acid to make the reaction slower. Fifth, the color being displayed can be adjusted by choosing different amino acids or amines. Sixth, the darkness of the color being displayed can be adjusted by the amount of the amino acids or amines.
Seventh, the assay is extremely easy to mn and interpret. And finally, the liquid transferring device could be used for any "fixed-volume" transfer in chemistry, biochemistry, clinical chemistry or other industries.
EXAMPLES
Example 1. Effect of OPA to Sodium Bisulfate mole ratio (0.5:1 to 8:1) Sodium bisulfate, glycine and OPA were added in sequence. The OPA to sodium bisulfate mole ratio was adjusted from 0.5:1 to 8:1 (Table 1). Table 1 shows that the solution with a 2:1 ratio developed a color while a 1:1 ratio did not show color in one week.
It was found that less than the theoretical amount of sodium bisulfate was needed to react with the OPA. This indicates the OPA solutions in this concentration region can be differentiated by observing the color of the solution after a specified time (as in Vial 2 and Vial 3). Since we can control the volume of OPA in testing, we can theoretically test an OPA solution in any concentration range.
Table 1.
Vial Vial Vial 3 Vial Vial l 2 4 s NaHSO; (82mM) 200p,1 200p,1 200p.1 200p,1 200p1 (0.0164 (0.0164 (0.0164 (0.0164 (0.0164 mMole) mMole) mMole) mMole) mMole) Glycine (82mM) 1600pL 1600p,L 1600pL 1600pL 1600pL
(0.1312 (0.1312 (0.1312 (0.1312 (0.1312 mMole) mMole) rnMole) mMole) mMale) OPA (0.55%, 4lmM)200pL 400p,L 800~tL 1600~L 3200~rL
(0.00820(0.0164 (0.0328 (0.0656 (0.1312 mMole) mMole) mMole) mMole) mMole) OPA:NaHS03 mole 0.5:1 1:1 2:1 4:1 8:1 ratio Tirne to develo > 1 week> 1 week4' 45" 65" 35"
color Initial color ColorlessColorlessLi ht e1/ ellow/arne1/ rn rn Final color (afterColorlessColorlessDark reen Between Dark 30') Blck Example 2. Effect of OPA to Sodium Bisulfate mole ratio (1:1 to 2:1).
Sodium bisulfate, glycine and OPA were added and the OPA to sodium bisulfate mole ratio was adjusted as in Example 1. Table ? shows three points of interest (POI).
The first POI, was the 2:1 mole ratio, the second POI was the 1.75:1 mole ratio and the third POI was the 1.5:1 mole ratio of OPA to sodium bisulfate. For the 2:1 ratio, 5 minutes were needed to display the initial color. For the 1.75:1 ratio, 13 minutes were needed to display the initial color. For the 1.5:1 ratio, color was not displayed for a few days.
Table 2.
Vial Vial Vial Vial 4 Vial s l 2 3 NaHS03 (82mM) 200p1 200111 200p1 200y1 200p1 (0.0164(0.0164(0.0164(0.0164 (U.0164 mMole) mMole) mMole) mMole) mMole) Glycine (82mM) 1600~L 1600~L 1600~,L1600YL 160Up.L
(0.1312(0.1312(0.1312(0.1312 (0.1312 mMole) mMole) mMole) mMole) mMole) OPA (0.55%, 4lmM)400ftL SOONL 600ttL 700p,L 8001.tL
(0.00164(U.0205(0.0246(0.0278 (0.0328 mMole) mMole) mMole) mMole) mMole) OPA:NaHSO, mole ratio 1:1 1.25:1 1.5:1 1.75:1 2:1 Time to develo Never Never Never 13' S' color Initial color ColorlessColorlessColorlessVery light(Light) Pink YellGrn Final color (afterColorlessColorlessColorlessGreen Dark Grn 30') In Table 2, the reaction volume is varied by varying the amount of OPA
solution from 400 ,u1 to 800 ,u1. The asscry is independent of volume. The OPA to sodium bisulfite mole ratio is a key parameter of the assay.
Example 3. OPA Concentration Variation Study in the OPA to Sodium Bisulfite Mole Ratio 1:1 to 2:1 Region. (same volume different concentration) Sodium bisultite, glycine and OPA were added and the OPA to sodium bisultite mole ratio was adjusted as in Example 2. As shown in Table 3> the tirst POI
was in the range of 6'20"-7'20" range and the time needed for color change was very consistent.
l5 However, for the second POI, there was some variation for this time (17-24'). Without being bound by any mechanism, this may be due to the visual limitation or it may mean that at diluted concentration, the color development is more likely to be influenced by micro reaction condition variations, such as temperature, pH or even the exposure of sunlight.
Table 3.
Vial Via12 Vial Vial Vial l 3 4 s NaHSO; (82mM') 200p,12001 2001 200p,1 200p1 (0.0164(0.0164 (0.0164(0.0164(0.0164 mMole)mMole) mMole) mMole) mMole) Glycine (82mM) 1600PL1600yL 1600~L 1600~L 160UpL
(0.1312(0.1312 (0.1312(0.1312(0.1312 mMole)mMole) mMole) mMole) mMole) OPA ( % ) 0.275 0.344 0.413 0.481 0.550 (20.50(25.63 (30.75 (35.88 (41.00 mM) mM) mM) mM) mM) ml (0.55%OPA) to dilute50.00 62.50 75.00 87.50 No to 100m1 with water dilution OPA solution used 800p,18001 8001 8001 800p1 OPA mMole 0.01640.0205 0.0246 0.0287 0.0328 OPA:NaHS03 mole ratio1:1 1.25:1 1.5:1 1.75:1 2:1 Time to develop colorNever Never Never 17-- 6' 20"
20' --7' 20"
Time to develop color,Never Never Never 18-- 6' 20"
repeat 21' --7' # 1 20"
Time to develop color,Never Never Never 19-- 6' 20"
repeat 21' --7' #2 20"
Time to develop color,Never Never Never 21-- 6' 20"
repeat 23' --7' #3 20"
Tirne to develop color,Never Never Never 22-- 6' 20"
repeat 24' --7' #4 20"
Initial color ColorlessColorlessColorlessVery (Light) light Yel/Grn ink Final color (after ColorlessColorlessColorlessDark Dark 2h) Grn Grn Example 4. OPA Concentration Variation Study Sodium bisulfite, glycine and OPA were added as in Example 1. Since the POI
position is controlled by the OPA to sodium bisultite mole ratio, by changing the OPA
volume, one should be able to switch the POI to basically any OPA
concentration range. Thus, in Table 4, the actual OPA moles taken in Vial 1, Vial 2 and Vial 3 are equal to Vial 3, Vial 4 and Vial 5 in Table 3.
Table 4.
Vial l Vial2 Vial3 NaHSO~ (82mM) 2001r1 200,1 200p.1 (0.0164 (0.0164 mMole)(0.0164 mMole) mMole) Glycine (82mM) 1600~L 1600p,L 1600~rL
(0.1312 (0.1312 mMole)(0.1312 mMole) mMole) OPA (%, 41m1VI) 0.275 0.344 0.413 ml (0.55~7oOPA) to 50.00 62.50 75.00 dilute to I OOmI
OPA solution used 12011 1119p,1 1065p1 (0.0246 (0.0287 mMole)(0.0328 mMole) mMole) OPA:NaHSO~ mole ratio1.5:1 1.75:1 2:1 Time to develop colorNever 16' S' (up to 30' ) Initial color Colorless (1i ht) Yel/Grn(La ht) Yel/Grn Thus, one of the key factors for this invention is the mole ratio of aldehyde to sodium bisulfate. Similar results were obtained for Dr.-alanine, s-amino-n-caproic acid and L-lysine, except that different end colors were observed.
Example 5: Further experiments with OPA for POI's in the range of 0.35 % and 0.30 % .
Changes due to the type of amino acid and the mole ratio were illustrated in the following example where DL-dopa is used as the amino acid (also see Example 7).
Sodium bisulfate, and OPA were added as in Example 1. DL-dopa was substituted for glycine as the amino acid.
Table 5.
82mM NaHS03 Saturated0.35% OPA 0.30% 0.35% OPA 0.30% OPA
OPA
or.-dope(23.09rnM)(22.37mM)(23.09mM) (22.37mM) Color in Color in (minutes (minutes and and seconds) seconds) 1001 100u1 4501 4501 2'20"-2'30" 3'20"-4' (0.0082mMole) (0.0119 ('0.0101 mMole) mMole) 100p1 1001 400p1 400p1 3'00"-3'30" 5'-10' (0.0082mMole) (0.0106 (0.0089 mMole) mMole) 100p1 1001 390y1 390p1 3'40"-4'10" 5'30"-11' (0.0082mMole) (0.0103 (0.0087 mMole) mMole) In the above example, the use of ~L-dope as the amine resulted in an orange color. The type of amino acid, mole ratio, and reaction time are all important to determine the formation of color.
Example 6. Base Effect for the Color Development Time.
This example shows that added base promotes the reaction rate so that the color displaying time can be shortened. Thus, a certain amount of base could be added to display the color within a desired period of tune.
Table 6.
Vial1 Vial2 Vial3 Vial4 NaHSO~ (82mM) 200~t1 200~t1 200p1 200~t1 (0.0164 (0.0164 (0.0164(0.0164 mMole) mMole) mMole) mMole) Glycine (82mM) 1600pL 1600~tL 16001tL1600p,L
(0.1312 (0.1312 (0.1312(0.1312 mMole) mMole) mMole) mMole) OPA ( % ) (variation 0.275 0.344 0.413 0.481 cone) ml (O.SS~oOPA), added 50.00 62.50 75.00 87.50 to dilute to 100m1 OPA (0.5510, 4lmM)(initial800p1 800~t1 8001 800p.1 cone) (0.0164 (0.0205 (0.0246(0.0287 mMole) mMole) mMole) mMole) OPA:NaHSO~ mole ratio 1:1 _ 1.25:1 1.5:1 1.7_5:1 _ __ Time to develop color colorlesscolorlesscolorlessVery light (without NaOH) _ I ink (17'-24') Time to develop color 1.5h slight1h slight2' yellow<2', yellow (100pL
NaOH added) yellow yellow Time to develop color All turned (200f.tL yellow in less than 1'. Too fast.
Too NaOH added) much base.
Note: Sodium hydroxide was added before OPA.
Conversely, it was found that added acid, such as citric acid, would delay the color display. This would be useful in the case if the color is displayed too soon (data not shown).
Example 7. Other Amino Acids with Added Base (100pL).
It was found with other amino acids that the displayed colors were different.
For example, when reacting with OPA, D1.-alanine was bright yellow and for E-arnino-n-caproic acid, the color was pink. Furthermore, the reaction rates were also different.
Thus both DL-alanine and s-amino-n-caproic acid displayed color' significantly later than glycine (data not shown).
Example 8. Activated Cidex solution (containing 2.1 % glutaraldehyde) with Lysine To five scintillation vials, glutaraldehyde, sodium bisulfate and lysine were added and mixed. A yellow color developed gradually from Vial 5. No color was observed in Vial 1. The "between" colors were seen from Vial 2 to Vial 4 but they are so "gradual" that they could not be distinguished visually.
Table 7.
Vial l Vial Vial3 Vial Vial s -_- -- ?~O~cl 2~O,ul ZOO,tal ?OOfcl ?~l)~cl NaHS03 (82 mM) _____ (0.0164 (0.0164(0.0164 (0.0164 (0.0164 mMole) mMole) mMole) mMole) mMole) Lysine (82mM) 1600 ,u1 1600 1600 1600 1600 ,ccl fcl ,ccl )c1 (0.1312 (0.1312(0.1312 (0.1312 (0.1312 mMole) mMole) mMole) mMole) mMole) Glutaraldeyde (220mM) solution74.5 ,ccl93.2 111.8 130.5 149.1 used ,ecl ,ecl u1 ,ccl (0.0614 (0.0205(0.0246 (0.0287 (0.0328 mMole) mMole) mMole) mMole) mMole) Glutaraldehyde:NaHSO~ mole 1:1 1.25:1 1.5:1 1.75:1 2:1 ratio ~ _ ~__ _ _- ColorlessVery Yellow Color at 15 minutes light yellow to yellow, very gradual.
No clear-cut difference This can be explained in light of the stabilities of the compounds involved.
First, if aldehyde-sodium bisulfite complex 5 is more stable than aldehyde-sodium bisulfite complex 6, we would see a larger POI range from glutaraldehyde.
OH OH
~S03Na ~SU~Na S03Nat S03Na OH OH
(Colorless) (Colorless) 1 ~ More Sable Less Stahle The Ranges of POI Are Related to the Stability of Compound 5 and 6.
Or in more accurate terms, the different POI ranges from OPA and glutaraldehyde might be a result of the competence of aldehyde-sodium bisulfate formation and the aldehyde/amino acid Schiff s base formation both kinetically and thermodynamically.
()H
Routc L: So,Na NaHS()a ~ O SO;Na O
OH
O wH S
H (Cohxlcss) L (OI'AI
N Hz ~N ~-C()OH
~ Stability:5»>7 ~N L()()H
7 NHz (Ytllow) ()H
Routc 2:
'SO~Na NaHSOa ~ SO~Na O
H fi ()H
H (('e~larlessl l.) sittC
R ((~lutualdchydcl\
N HZ
N ~C O()H
Stabilit :6>9 N C:()OH
(Yellow) In Route 1, when the three components are mixed together, the formation of compound 5 is more favorable than the formation of compound 7, both kinetically and thermodynamically.
This is somewhat different in the situation of Route ?. Although the formation of 6 is still more favorable than that of 9, the difference is much smaller than that between 7 and 5 in Route 1. Therefore if the three components (glutaraldehyde, sodium bisulfite and lysine) are mixed, depending on the ratio, there tnay be some small amount of 9 formed which results in a detectable yellow color. However, this situation is manipulated by mixing of compound 8 and NaHSO; first and adding lysine last.
In this I S case, if there is no aldehyde left, lysine must compete with 6 to form 9, which is not very favorable. With some combinations of amino acid and aldehyde, the order of adding the reactants may be important. In the following example, the amino acid was added last.
Example 9. Amino acid was added last To five scintillation vials, glutaraldehyde and sodium bisulfite were added and mixed first, and lysine solution was added last respectively. A yellow color developed gradually from Vial 5 to Vial 2 but not in Vial 1 (Table 8).
Table 8.
__ Vial Vial Vial Vial Vial l 2 3 4 s ~OOp.I 200p.1 2001 200p,1200p,1 aHSO, (82mM) (0.0164(0.0164(0.0164('0.0164(0.0164 _______ ___ rnMole)_Mole) Mole) Mole) Mole) 1600p.L1600pL 1600yL 1600yL1600~L
ysine (82mM) (0.1312(0.1312(0.1312(0.1312(0.1312 _ mMole) mMole) mMo_le)mMole)Mole) _ lutaraldehyde (220mM) 4.51 3.2p1 111.8,1130.Sp,l149.11 solution sed (0.0614(0.0205(0.0246(0.0287(0.0328 mMole) mMole) Mole) nMole)mMole) lutaraldehyde: ! NaHSO, mole atio 1:1 1.25:1 1.5:1 1.75:1~:l _-____-__. _ __ _ __ _ r~ht olor at 15' olorlessellow ellow ellow ellow A narrower POI range was observed for glutaraldehyde reacting with lysine and sodium bicarbonate. Adding the amino acid (lysine) last was the key. Table 8 shows a clear color difference between Vial 1 (color less) and Vial 3 (yellow). Thus by allowing the glutaraldehyde and sodium bisultite to react first and then adding lysine, results are similar to those observed with OPA above.
Depending on the chemicals used, the time may vary. For NaHS03, the lysine can be added immediately after the aldehyde is mixed with the NaHSOj. Thus the assay described can be applied generally to aldehydes and amines to provide a pass/fail type assay of aldehyde content.
Example 10.
The above chemistry principle may be applied in the reaction of aldehydes and compounds containing an amino group generally. This example shows the reaction of glutaraldehyde and sodium cyanide using either glycine or lysine as the amino acid.
The formation of corresponding two aldehyde cyanide addition compounds are shown as below.
-2 l 0 off H NaC'~ ON
H
U 10 ()H
1 (OI'Ai (Colorless) () ()H
H 'Yak C N
H ('N
() 11 OH
8 ((ilutaraldehydc) (Colorless) The Formation of Colorless Aldehyde-Cyanide Addition Compounds 10 and 11 To each of the _5 scintillation vials, glutaraldehyde and sodium cyanide were added and mixed first (Table 9), and lysine solution was added last. A yellow color developed from Vial 5 but not from the other vials. A POI was identified between Vial 4 and Vial 5.
Table 9.
Glutaraldehvde : Sodium Cyanide Mole Ratio (0.125:1 to 2:1 ).
Viall Vial2 Vial3 Vial4 ial5 OOp.I 2001 200p,1 ~00~1 ~OOpI
aCN (82mM) (0.0164(0.0164(0.0164 (0.0164 (0.0164 _____ rnMo_le)Mole) rnMole)mMole) mMole) 1600pL1600~rL1600~L 1600~rL 1600~,L
lycine (82mM) (0.1312(0.13120.1312 0.1312 (0.1312 _ Mole) Mole) mMole) mMole)_ Mole) .31.11I 8.6p137.3p1 4.5p,1 149.1 p.1 lutaraldehyde (220mM) (0.0020(0.0041(0.00820.0164 0.0328 solution sed mMole)mMole) Mole) mMole) mMole) lutaraldeh de:NaCN mole _.125:125:1 .5:1 l :l 2:1 ratio olorles Final color in 7' _-~_ ~-- olorlessolorlessColorlessYellow , Example 11 To each of the 5 scintillation vials, glutaraldehyde and sodium cyanide were added and mixed first, and lysine solution was added last (Table 10). A yellow color developed from Vial 2 to Vial 5 but not recognizable from Vial 1. A POI was identified between Vial 1 and Vial 3. It is only practical with the naked eye to differentiate the colors between Vial I and Vial 3. That is, it would be challenging to distinguish the difference between Vial 1 and Vial 2 or between Vial 2 and Vial 3.
Thus we may conclude that no narrower POI could be identified unless an instrument is employed.
Table 10.
Glutaraldehyde : Sodium Cyanide Mole Ratio ( 1:1 to 2:1 ).
__ _ Via_I Vial 2 Vial Vial _Vi_al I_ 3 4 5 200u1 200p1 200P1 200p1 200y1 NaCN (82mM) (0.0164 (0.0164 (0.0164 (0.0164 (0.0164 _ _ mMole) mMole) mMole) mMole) mMole) 1600yL 1600p.L 1600p.L 1600~L 1600~.L
Glycine (82mM) (0.1312 (0.1312 (0.1312 (0.1312 (0.1312 mMole) mMole) mMole) mMole) mMole) 93.21 149.1 p1 74.5p.1 111.8~ 130.51 Glutaraldehyde (0.0164 (0Ø.05 ~ (0.0164 (0.0328 ~ (0.008:.
(220mM) solution mMolej mMole) mMole) mNtole) mMole) used _ _ Glutaraldehyde:NaCN1;1 1.25:1 1.5:1 1.75:1 2:1 mole ratio ' Time to develo Never 3' 2' ~ 1' 1' color Color in ~8 minutes Very light Colorless yellow Yellow Yellow Yellow The aldehyde solution can be measured and transferred by means known in the art such as by a regular pipet or syringe. In a preferred embodiment, the aldehyde solution can be measured and transferred using a liquid measuring device as described herein which features a gas or vapor permeable, liquid impermeable, membrane.
The use of the liquid measuring device containing the gas or vapor permeable, liquid impermeable membrane of the present disclosure has the advantage that the liquid can be transferred easily using a simple operation with consistent results.
Compound X and Compound Y (Figure 1) may be in one vial or in two separate 1 ~ vials. Thev may be transferred using either a pipet or syringe. The aldehyde may be added to compound X and the resulting mixture added to compound Y, the aldehyde may be added to compounds X and Y together, or the aldehyde and chemical Y can be added to the chemical X consecutively. The measuring and/or transferring of the aldehyde test sample can be conducted with a regular pipet or syringe. The gas or vapor permeable liquid impermeable barner adds many benefits as described previously.
In one embodiment, shown in Figure 6C, the Compound X may be in a first chamber 9. The aldehyde is drawn up through the valve 8 up to the gas or vapor permeable, liquid impermeable barner 1. After a predetermined time, the aldehyde and compound X are transferred to a second chamber 10 through a valve 8 which is either a one-way or an on/off valve, where they react with compound Y. After a pre-determined time, the color in the second chamber is observed and the presence or absence of excess aldehyde in the test sample is determined.
It will be understood by those of skill in the art that numerous and various modifications can be made without departing from the spirit of the present invention.
Therefore, it should be clearly understood that the forms of the present invention are illustrative only and are not intended to limit the scope of the present invention.
_~5_
In a preferred embodiment, the method further includes adjusting the position of the barrier in the barrel. In a preferued embodiment, the barrier is part of a coupling device and the method further includes adapting the coupling device to the barrel. In a more preferred embodiment, the adapting includes inserting the coupling device into ?5 the barrel.
In a preferred embodiment, the barrel further includes a valve at the distal end and the method further includes opening and/or closing the valve.
In a preferred embodiment, the method further includes pulling a plunger in the barner to create a negative pressure.
For purposes of summarizing the invention and the advantages achieved over the prior art, certain objects and advantages of the invention have been described above. Of course, it is to be understood that not necessarily all such objects or advantages may be achieved in accordance with any particular embodiment of the invention. Thus, for example, those skilled in the art will recognize that the invention may be embodied or carried out in a manner that achieves or optimizes one advantage or group of advantages as taught herein without necessarily achieving other objects or advantages as may be taught or suggested herein.
Further aspects, features and advantages of this invention will become apparent from the detailed description of the preferred embodiments which follow.
Brief Description of the Drawings These and other feature of this invention will now be described with reference to the drawings of preferred embodiments which are intended to illustrate and not to limit the invention.
Figure 1 shows the basic principles of the described assay. Reaction 1 shows the reaction of aldehyde with compound X to produce a compound with a first color.
Preferably, the first color is colorless. Reaction ? shows the reaction of aldehyde and Y
to form a compound with a second color. Preferably, reaction 2 is slower than Reaction 1. If the concentration of aldehyde is below the POI (point of interest) only compound X will react and the resulting solution will be the first color as shown in the bottom half ?0 of the figure. In the presence of a level of aldehyde that is equal to or more than the PUI, a solution with the second color or the combined color of the first color and the second color will be formed.
Figure ? shows a pipette and two variants of a syringe with a gas or vapor permeable liquid impermeable barrier.
Figure 3A shows the coupling of the gas or vapor permeable liquid impermeable barrier to the syringe or pipette. Figure 3B illustrates how inserts 4 at the top of the pipette or syringe attach the gas or vapor permeable liquid impermeable barrier to the pipette or syringe. Figure 3C illustrates a holder 5 that holds the inserts in place.
Figure 3D shows the inserts and the coupling of the gas or vapor permeable liquid impermeable barrier.
Figure 4 is an expanded view of figure 3C which shows a gas or vapor permeable liquid impermeable barner l, an insert 4, and a holder 5.
Figure 5 shows one embodiment of the invention where the position of the gas or vapor permeable liquid impermeable membrane is adjusted by means of a screw.
Figures 6A and 6B show embodiments of the liquid delivery apparatus with all chemicals in one chamber. Figure 6C shows a two chambered embodiment of the liquid delivery apparatus. The test sample may be taken into the first chamber for reaction with the first compound such as compound X in Figure 1. Then the sample is moved by means of a one-way valve or a manual ON/OFF valve 8 into the second chamber where the test sample reacts with the second compound such as compound Y
of Figure 1.
Detailed Description of the Preferred Embodiment While the described embodiment represents the preferred embodiment of the present invention, it is to be understood that modifications will occur to those skilled in the art without departing from the spirit of the invention. The scope of the invention is therefore to be determined solely by the appended claims.
Aldehydes react with amino-containing compounds like amino acids or amines to form an imine or more commonly known as a Schiff's base, which is often colored.
Taking glycine as an example:
p N
() ~ ~--()H
~H ~ O
? H=N () H ~<>ri (>H
() r ? 3 ((srecn to r3lack, changine Irom li~~hter to darker) Schiff's Base Formation between OPA and Glycine Another known aldehyde reaction is the sodium bisulfate carbonyl addition reaction.
O UH
H ~ ~ ~SO;Na + 2 NaHSO; SOjNa H
O OH
t a (Colol'Iess) Addition Reaction of Sodium Bisulfate to OPA
The sodium bisulfate addition reaction is more favorable than that of Schiff's formation since the former reaction is fast and hard to reverse. Thus, in the presence of both a compound containing an amino group such as an amino acid and a reagent such as sodium bisulfate, the aldehyde will react first with sodium bisulfate and then with the amino acid. Therefore, it is possible to design a color pass/fail reaction by controlling the amount of reagents to react with aldehydes such as formaldehyde, OPA or glutaraldehyde. The key is the amount of reagent such as sodium bisulfate which is designed to react with the aldehyde without a color being developed in the presence of I S an amino acid. Any remaining aldehyde will then react with the amino acid to develop a colored solution. This confirms the presence of a certain amount of an aldehyde such as formaldehyde, OPA or glutaraldehyde in a test solution such as a disinfectant solution. On the other hand, if no color was developed, it confirms that the formaldehyde, OPA or glutaraldehyde concentration is below an acceptable specitication. The specific concentration can be set to any point by adjusting the amounts of the chemical reagents used or by using different amounts of aldehyde (formaldehyde, OPA or glutaraldehyde) in the test solution.
Thus, a color pass/fail reaction for determination of excess aldehyde by control of reagents which react with aldehyde is described. The key is the amount of reagent ?5 such as sodium bisulfate which is designed to react with the Point of Interest (POI) level of aldehyde without a color being developed in the presence of a compound containing an amino group such as an amino acid. Any ''extra" aldehyde, exceeding the POI, will then react with the compound containing an amino group, causing a color to be developed. In a preferred embodiment, the aldehyde is either OPA or glutaraldehyde and the compound containing the amino group is an amino acid. This method is especially useful for quality control where components only needed to be examined in pre-determined ranges.
A number of reagents which are known to react quickly with aldehydes may be used in the practice of the invention. These include any chemicals which can oxidize or reduce the aldehyde group and any chemicals which can react with and alter the carbonyl functional group of the aldehyde. Examples of such reagents are disclosed in Morrison & Boyd, "Organic Chemistry", Chapter 19, Allyn and Bacon, 3"~
edition, 1973, which is herein incorporated by reference. Such reagents include, but are not limited to, Ag(NH3)~; KMnO~; K,Cr~O~; H, + Ni, Pt, or Pd; LiAIHa or NaBH.~, then H+;
Zn (Hg), conc. HCI; NH~NHZ, base; Grignard reagents; salts of cyanide and bisulfite;
ammonia derivatives such as hydroxylamine, hydrazine, phenylhydrazine, and semicarbazide; reactions with alcohols in the presence of acid; and reactions with acid or base such as the Cannizzaro reaction, the aldol condensation, and the Perkin condensation. In a preferred embodiment, the reagent which reacts with the aldehyde is a salt of either bisulfite or cyanide.
This aspect of the invention is illustrated in Figure 1. Both compounds X and Y react with the aldehyde in the figure. Preferably X reacts much faster than Y.
?0 Preferably, the reaction of X with aldehyde results in a colorless compound whereas the reaction of Y with aldehyde results in a colored compound. A point of interest is chosen and the amount of X that will react with the point of interest is determined.
When the aldehyde is mixed with X and Y, the aldehyde will react first with compound X which is kinetically and thermodynamically favored. Any excess aldehyde will then react with compound Y to form a colored solution.
Consequently, if a colored solution results, the concentration of aldehyde is above the point of interest. The determination may be made visually, with or without a color chart.
Alternatively, a spectrophotometer may be used. If the reaction between the aldehyde and compound X is not kinetically and thermodynamically favored, then compound Y
can be added after the aldehyde reacts with compound X as shown in Figure 1.
_7_ The theoretical amount of OPA: sodium bisulfate is I :2. However, it was found that less sodium bisulfate is needed to react with OPA than the theoretical amount in order to get a good color display.
Another aspect of the invention is a liquid-measuring device, such as a pipette or syringe, for carrying out the assay. This device could be used for any "faxed-volume" measurement and transfer in chemistry, biochemistry, clinical chemistry or other industries.
The apparatus may be a syringe or pipette with one or more barrels and plungers and a membrane barrier with or without a coupling device. The membrane barrier is a gas or vapor permeable and liquid impermeable barrier. In the presence of certain pressure differences between the two sides of the barrier, the gas or vapor flows through the membrane but not the liquid. Any suitable gas or vapor permeable and liquid impermeable materials can be used for this purpose. Some examples include, but are not limited to, nonwoven polyolefin, such as Tyvek~a~~a (non-woven polyethylene), or CSR (non-woven polypropylene central supply room), wrapping material and any other hydrophobic filtering materials. Optionally, the device contains an insert and a holder.
The syringe or pipette apparatus may also contain valves to control the flow of liquid.
The membrane barrier can be thermally bound to the syringe or pipet. It can also be attached to the syringe or pipet with an adhesive or connected to the syringe barrel by a coupling device. The coupling device may be connected to an insert for altering the position of the membrane barrier. The position of the membrane barrier can be adjusted by the length of the insert. The insert may be secured with a holder.
The membrane barner is a gas or vapor permeable but liquid impermeable barrier. The membrane barrier is positioned such that the liquid can only be tilled up to the barrier. The invention has several preferred embodiments.
In the first embodiment (Figure 2), a gas or vapor permeable liquid impermeable membrane 1 is fixed into the pipette 7 or syringe 6 and held in place at the desired maximum volume by means known in the art. The syringe includes a plunger 3.
The syringe can have a metal or plastic needle with or without a needle cap. In one embodiment (Figures 3A-3D), a coupling device 2 is used which is larger or smaller _g_ than the diameter of the pipette 7 or syringe 6. Two parts of the pipet or syringe with different lengths can be joined together with such a coupling device.
Coupling of the membrane barrier to the syringe or pipette is shown in Figures 3A, 3B, 3C, 3D and Figure 4. The membrane can be inserted into the syringe or pipet from the top of the pipette or syringe by an insert 4 which may be secured with a holder 5 and its position varied by any means known in the art such as by a screw (Figure 5) or a slidable adjustment (Figure 4j. Figure 3D shows an insert which has a larger diameter than the pipette or syringe. By adjusting the insert and creating a negative pressure on the upper part of the pipette or syringe, the fluid can be loaded into the syringe or pipette up to the barrier.
Figures 6A, 6B and 6C illustrate the use of the measuring device with this invention. Figures 6A and 6B show a syringe with a gas or vapor permeable liquid impermeable barrier and two chemicals. The liquid can be filled in the syringe by inserting the plastic needle into the sample solution, pulling the plunger to create a negative pressure in the syringe, and loading the liquid into the syringe. The measuring device can have a filtering material (Figure 6A) or valve (Figure 6B) to retain the chemicals in the barrel. The chemical in the syringe can be in either a liquid or solid form. The valve can be a one-way valve or a manual ON/OFF valve.
Figure 6C provides another embodiment for mixing more than one reactant successively. It has two chambers 9, 10. A fixed volume of any solution including, but not limited to an aldehyde is drawn up through a one-way valve or an ON/OFF
valve 8 into the first chamber 9 where it mixes with the first reactant, for example sodium bisulfite. After a predetermined time, the reactants flow through a second one-way valve or an ONIOFF valve 8 into a second reaction chamber 10 which might contain an amine such as lysine, for example, to complete the reaction.
Alternatively, a three-way valve can be used instead of two one-way valves.
The invention has several advantages over the prior art methods. First, the pass/fail conclusion is consistent and convenient. Preferably, there is no need to guess the color. The user's only conclusion will be "colored" or "not colored."
Second, the liquid transferring device is consistent and convenient. A fixed volume of liquid can be taken by a simple operation. Third, the solution color is easier to visualize than a test strip paper since the test strip paper itself is colored, leading to false positive results.
Fourth, the color displaying time can be adjusted by adding a base to make the reaction faster or an acid to make the reaction slower. Fifth, the color being displayed can be adjusted by choosing different amino acids or amines. Sixth, the darkness of the color being displayed can be adjusted by the amount of the amino acids or amines.
Seventh, the assay is extremely easy to mn and interpret. And finally, the liquid transferring device could be used for any "fixed-volume" transfer in chemistry, biochemistry, clinical chemistry or other industries.
EXAMPLES
Example 1. Effect of OPA to Sodium Bisulfate mole ratio (0.5:1 to 8:1) Sodium bisulfate, glycine and OPA were added in sequence. The OPA to sodium bisulfate mole ratio was adjusted from 0.5:1 to 8:1 (Table 1). Table 1 shows that the solution with a 2:1 ratio developed a color while a 1:1 ratio did not show color in one week.
It was found that less than the theoretical amount of sodium bisulfate was needed to react with the OPA. This indicates the OPA solutions in this concentration region can be differentiated by observing the color of the solution after a specified time (as in Vial 2 and Vial 3). Since we can control the volume of OPA in testing, we can theoretically test an OPA solution in any concentration range.
Table 1.
Vial Vial Vial 3 Vial Vial l 2 4 s NaHSO; (82mM) 200p,1 200p,1 200p.1 200p,1 200p1 (0.0164 (0.0164 (0.0164 (0.0164 (0.0164 mMole) mMole) mMole) mMole) mMole) Glycine (82mM) 1600pL 1600p,L 1600pL 1600pL 1600pL
(0.1312 (0.1312 (0.1312 (0.1312 (0.1312 mMole) mMole) rnMole) mMole) mMale) OPA (0.55%, 4lmM)200pL 400p,L 800~tL 1600~L 3200~rL
(0.00820(0.0164 (0.0328 (0.0656 (0.1312 mMole) mMole) mMole) mMole) mMole) OPA:NaHS03 mole 0.5:1 1:1 2:1 4:1 8:1 ratio Tirne to develo > 1 week> 1 week4' 45" 65" 35"
color Initial color ColorlessColorlessLi ht e1/ ellow/arne1/ rn rn Final color (afterColorlessColorlessDark reen Between Dark 30') Blck Example 2. Effect of OPA to Sodium Bisulfate mole ratio (1:1 to 2:1).
Sodium bisulfate, glycine and OPA were added and the OPA to sodium bisulfate mole ratio was adjusted as in Example 1. Table ? shows three points of interest (POI).
The first POI, was the 2:1 mole ratio, the second POI was the 1.75:1 mole ratio and the third POI was the 1.5:1 mole ratio of OPA to sodium bisulfate. For the 2:1 ratio, 5 minutes were needed to display the initial color. For the 1.75:1 ratio, 13 minutes were needed to display the initial color. For the 1.5:1 ratio, color was not displayed for a few days.
Table 2.
Vial Vial Vial Vial 4 Vial s l 2 3 NaHS03 (82mM) 200p1 200111 200p1 200y1 200p1 (0.0164(0.0164(0.0164(0.0164 (U.0164 mMole) mMole) mMole) mMole) mMole) Glycine (82mM) 1600~L 1600~L 1600~,L1600YL 160Up.L
(0.1312(0.1312(0.1312(0.1312 (0.1312 mMole) mMole) mMole) mMole) mMole) OPA (0.55%, 4lmM)400ftL SOONL 600ttL 700p,L 8001.tL
(0.00164(U.0205(0.0246(0.0278 (0.0328 mMole) mMole) mMole) mMole) mMole) OPA:NaHSO, mole ratio 1:1 1.25:1 1.5:1 1.75:1 2:1 Time to develo Never Never Never 13' S' color Initial color ColorlessColorlessColorlessVery light(Light) Pink YellGrn Final color (afterColorlessColorlessColorlessGreen Dark Grn 30') In Table 2, the reaction volume is varied by varying the amount of OPA
solution from 400 ,u1 to 800 ,u1. The asscry is independent of volume. The OPA to sodium bisulfite mole ratio is a key parameter of the assay.
Example 3. OPA Concentration Variation Study in the OPA to Sodium Bisulfite Mole Ratio 1:1 to 2:1 Region. (same volume different concentration) Sodium bisultite, glycine and OPA were added and the OPA to sodium bisultite mole ratio was adjusted as in Example 2. As shown in Table 3> the tirst POI
was in the range of 6'20"-7'20" range and the time needed for color change was very consistent.
l5 However, for the second POI, there was some variation for this time (17-24'). Without being bound by any mechanism, this may be due to the visual limitation or it may mean that at diluted concentration, the color development is more likely to be influenced by micro reaction condition variations, such as temperature, pH or even the exposure of sunlight.
Table 3.
Vial Via12 Vial Vial Vial l 3 4 s NaHSO; (82mM') 200p,12001 2001 200p,1 200p1 (0.0164(0.0164 (0.0164(0.0164(0.0164 mMole)mMole) mMole) mMole) mMole) Glycine (82mM) 1600PL1600yL 1600~L 1600~L 160UpL
(0.1312(0.1312 (0.1312(0.1312(0.1312 mMole)mMole) mMole) mMole) mMole) OPA ( % ) 0.275 0.344 0.413 0.481 0.550 (20.50(25.63 (30.75 (35.88 (41.00 mM) mM) mM) mM) mM) ml (0.55%OPA) to dilute50.00 62.50 75.00 87.50 No to 100m1 with water dilution OPA solution used 800p,18001 8001 8001 800p1 OPA mMole 0.01640.0205 0.0246 0.0287 0.0328 OPA:NaHS03 mole ratio1:1 1.25:1 1.5:1 1.75:1 2:1 Time to develop colorNever Never Never 17-- 6' 20"
20' --7' 20"
Time to develop color,Never Never Never 18-- 6' 20"
repeat 21' --7' # 1 20"
Time to develop color,Never Never Never 19-- 6' 20"
repeat 21' --7' #2 20"
Time to develop color,Never Never Never 21-- 6' 20"
repeat 23' --7' #3 20"
Tirne to develop color,Never Never Never 22-- 6' 20"
repeat 24' --7' #4 20"
Initial color ColorlessColorlessColorlessVery (Light) light Yel/Grn ink Final color (after ColorlessColorlessColorlessDark Dark 2h) Grn Grn Example 4. OPA Concentration Variation Study Sodium bisulfite, glycine and OPA were added as in Example 1. Since the POI
position is controlled by the OPA to sodium bisultite mole ratio, by changing the OPA
volume, one should be able to switch the POI to basically any OPA
concentration range. Thus, in Table 4, the actual OPA moles taken in Vial 1, Vial 2 and Vial 3 are equal to Vial 3, Vial 4 and Vial 5 in Table 3.
Table 4.
Vial l Vial2 Vial3 NaHSO~ (82mM) 2001r1 200,1 200p.1 (0.0164 (0.0164 mMole)(0.0164 mMole) mMole) Glycine (82mM) 1600~L 1600p,L 1600~rL
(0.1312 (0.1312 mMole)(0.1312 mMole) mMole) OPA (%, 41m1VI) 0.275 0.344 0.413 ml (0.55~7oOPA) to 50.00 62.50 75.00 dilute to I OOmI
OPA solution used 12011 1119p,1 1065p1 (0.0246 (0.0287 mMole)(0.0328 mMole) mMole) OPA:NaHSO~ mole ratio1.5:1 1.75:1 2:1 Time to develop colorNever 16' S' (up to 30' ) Initial color Colorless (1i ht) Yel/Grn(La ht) Yel/Grn Thus, one of the key factors for this invention is the mole ratio of aldehyde to sodium bisulfate. Similar results were obtained for Dr.-alanine, s-amino-n-caproic acid and L-lysine, except that different end colors were observed.
Example 5: Further experiments with OPA for POI's in the range of 0.35 % and 0.30 % .
Changes due to the type of amino acid and the mole ratio were illustrated in the following example where DL-dopa is used as the amino acid (also see Example 7).
Sodium bisulfate, and OPA were added as in Example 1. DL-dopa was substituted for glycine as the amino acid.
Table 5.
82mM NaHS03 Saturated0.35% OPA 0.30% 0.35% OPA 0.30% OPA
OPA
or.-dope(23.09rnM)(22.37mM)(23.09mM) (22.37mM) Color in Color in (minutes (minutes and and seconds) seconds) 1001 100u1 4501 4501 2'20"-2'30" 3'20"-4' (0.0082mMole) (0.0119 ('0.0101 mMole) mMole) 100p1 1001 400p1 400p1 3'00"-3'30" 5'-10' (0.0082mMole) (0.0106 (0.0089 mMole) mMole) 100p1 1001 390y1 390p1 3'40"-4'10" 5'30"-11' (0.0082mMole) (0.0103 (0.0087 mMole) mMole) In the above example, the use of ~L-dope as the amine resulted in an orange color. The type of amino acid, mole ratio, and reaction time are all important to determine the formation of color.
Example 6. Base Effect for the Color Development Time.
This example shows that added base promotes the reaction rate so that the color displaying time can be shortened. Thus, a certain amount of base could be added to display the color within a desired period of tune.
Table 6.
Vial1 Vial2 Vial3 Vial4 NaHSO~ (82mM) 200~t1 200~t1 200p1 200~t1 (0.0164 (0.0164 (0.0164(0.0164 mMole) mMole) mMole) mMole) Glycine (82mM) 1600pL 1600~tL 16001tL1600p,L
(0.1312 (0.1312 (0.1312(0.1312 mMole) mMole) mMole) mMole) OPA ( % ) (variation 0.275 0.344 0.413 0.481 cone) ml (O.SS~oOPA), added 50.00 62.50 75.00 87.50 to dilute to 100m1 OPA (0.5510, 4lmM)(initial800p1 800~t1 8001 800p.1 cone) (0.0164 (0.0205 (0.0246(0.0287 mMole) mMole) mMole) mMole) OPA:NaHSO~ mole ratio 1:1 _ 1.25:1 1.5:1 1.7_5:1 _ __ Time to develop color colorlesscolorlesscolorlessVery light (without NaOH) _ I ink (17'-24') Time to develop color 1.5h slight1h slight2' yellow<2', yellow (100pL
NaOH added) yellow yellow Time to develop color All turned (200f.tL yellow in less than 1'. Too fast.
Too NaOH added) much base.
Note: Sodium hydroxide was added before OPA.
Conversely, it was found that added acid, such as citric acid, would delay the color display. This would be useful in the case if the color is displayed too soon (data not shown).
Example 7. Other Amino Acids with Added Base (100pL).
It was found with other amino acids that the displayed colors were different.
For example, when reacting with OPA, D1.-alanine was bright yellow and for E-arnino-n-caproic acid, the color was pink. Furthermore, the reaction rates were also different.
Thus both DL-alanine and s-amino-n-caproic acid displayed color' significantly later than glycine (data not shown).
Example 8. Activated Cidex solution (containing 2.1 % glutaraldehyde) with Lysine To five scintillation vials, glutaraldehyde, sodium bisulfate and lysine were added and mixed. A yellow color developed gradually from Vial 5. No color was observed in Vial 1. The "between" colors were seen from Vial 2 to Vial 4 but they are so "gradual" that they could not be distinguished visually.
Table 7.
Vial l Vial Vial3 Vial Vial s -_- -- ?~O~cl 2~O,ul ZOO,tal ?OOfcl ?~l)~cl NaHS03 (82 mM) _____ (0.0164 (0.0164(0.0164 (0.0164 (0.0164 mMole) mMole) mMole) mMole) mMole) Lysine (82mM) 1600 ,u1 1600 1600 1600 1600 ,ccl fcl ,ccl )c1 (0.1312 (0.1312(0.1312 (0.1312 (0.1312 mMole) mMole) mMole) mMole) mMole) Glutaraldeyde (220mM) solution74.5 ,ccl93.2 111.8 130.5 149.1 used ,ecl ,ecl u1 ,ccl (0.0614 (0.0205(0.0246 (0.0287 (0.0328 mMole) mMole) mMole) mMole) mMole) Glutaraldehyde:NaHSO~ mole 1:1 1.25:1 1.5:1 1.75:1 2:1 ratio ~ _ ~__ _ _- ColorlessVery Yellow Color at 15 minutes light yellow to yellow, very gradual.
No clear-cut difference This can be explained in light of the stabilities of the compounds involved.
First, if aldehyde-sodium bisulfite complex 5 is more stable than aldehyde-sodium bisulfite complex 6, we would see a larger POI range from glutaraldehyde.
OH OH
~S03Na ~SU~Na S03Nat S03Na OH OH
(Colorless) (Colorless) 1 ~ More Sable Less Stahle The Ranges of POI Are Related to the Stability of Compound 5 and 6.
Or in more accurate terms, the different POI ranges from OPA and glutaraldehyde might be a result of the competence of aldehyde-sodium bisulfate formation and the aldehyde/amino acid Schiff s base formation both kinetically and thermodynamically.
()H
Routc L: So,Na NaHS()a ~ O SO;Na O
OH
O wH S
H (Cohxlcss) L (OI'AI
N Hz ~N ~-C()OH
~ Stability:5»>7 ~N L()()H
7 NHz (Ytllow) ()H
Routc 2:
'SO~Na NaHSOa ~ SO~Na O
H fi ()H
H (('e~larlessl l.) sittC
R ((~lutualdchydcl\
N HZ
N ~C O()H
Stabilit :6>9 N C:()OH
(Yellow) In Route 1, when the three components are mixed together, the formation of compound 5 is more favorable than the formation of compound 7, both kinetically and thermodynamically.
This is somewhat different in the situation of Route ?. Although the formation of 6 is still more favorable than that of 9, the difference is much smaller than that between 7 and 5 in Route 1. Therefore if the three components (glutaraldehyde, sodium bisulfite and lysine) are mixed, depending on the ratio, there tnay be some small amount of 9 formed which results in a detectable yellow color. However, this situation is manipulated by mixing of compound 8 and NaHSO; first and adding lysine last.
In this I S case, if there is no aldehyde left, lysine must compete with 6 to form 9, which is not very favorable. With some combinations of amino acid and aldehyde, the order of adding the reactants may be important. In the following example, the amino acid was added last.
Example 9. Amino acid was added last To five scintillation vials, glutaraldehyde and sodium bisulfite were added and mixed first, and lysine solution was added last respectively. A yellow color developed gradually from Vial 5 to Vial 2 but not in Vial 1 (Table 8).
Table 8.
__ Vial Vial Vial Vial Vial l 2 3 4 s ~OOp.I 200p.1 2001 200p,1200p,1 aHSO, (82mM) (0.0164(0.0164(0.0164('0.0164(0.0164 _______ ___ rnMole)_Mole) Mole) Mole) Mole) 1600p.L1600pL 1600yL 1600yL1600~L
ysine (82mM) (0.1312(0.1312(0.1312(0.1312(0.1312 _ mMole) mMole) mMo_le)mMole)Mole) _ lutaraldehyde (220mM) 4.51 3.2p1 111.8,1130.Sp,l149.11 solution sed (0.0614(0.0205(0.0246(0.0287(0.0328 mMole) mMole) Mole) nMole)mMole) lutaraldehyde: ! NaHSO, mole atio 1:1 1.25:1 1.5:1 1.75:1~:l _-____-__. _ __ _ __ _ r~ht olor at 15' olorlessellow ellow ellow ellow A narrower POI range was observed for glutaraldehyde reacting with lysine and sodium bicarbonate. Adding the amino acid (lysine) last was the key. Table 8 shows a clear color difference between Vial 1 (color less) and Vial 3 (yellow). Thus by allowing the glutaraldehyde and sodium bisultite to react first and then adding lysine, results are similar to those observed with OPA above.
Depending on the chemicals used, the time may vary. For NaHS03, the lysine can be added immediately after the aldehyde is mixed with the NaHSOj. Thus the assay described can be applied generally to aldehydes and amines to provide a pass/fail type assay of aldehyde content.
Example 10.
The above chemistry principle may be applied in the reaction of aldehydes and compounds containing an amino group generally. This example shows the reaction of glutaraldehyde and sodium cyanide using either glycine or lysine as the amino acid.
The formation of corresponding two aldehyde cyanide addition compounds are shown as below.
-2 l 0 off H NaC'~ ON
H
U 10 ()H
1 (OI'Ai (Colorless) () ()H
H 'Yak C N
H ('N
() 11 OH
8 ((ilutaraldehydc) (Colorless) The Formation of Colorless Aldehyde-Cyanide Addition Compounds 10 and 11 To each of the _5 scintillation vials, glutaraldehyde and sodium cyanide were added and mixed first (Table 9), and lysine solution was added last. A yellow color developed from Vial 5 but not from the other vials. A POI was identified between Vial 4 and Vial 5.
Table 9.
Glutaraldehvde : Sodium Cyanide Mole Ratio (0.125:1 to 2:1 ).
Viall Vial2 Vial3 Vial4 ial5 OOp.I 2001 200p,1 ~00~1 ~OOpI
aCN (82mM) (0.0164(0.0164(0.0164 (0.0164 (0.0164 _____ rnMo_le)Mole) rnMole)mMole) mMole) 1600pL1600~rL1600~L 1600~rL 1600~,L
lycine (82mM) (0.1312(0.13120.1312 0.1312 (0.1312 _ Mole) Mole) mMole) mMole)_ Mole) .31.11I 8.6p137.3p1 4.5p,1 149.1 p.1 lutaraldehyde (220mM) (0.0020(0.0041(0.00820.0164 0.0328 solution sed mMole)mMole) Mole) mMole) mMole) lutaraldeh de:NaCN mole _.125:125:1 .5:1 l :l 2:1 ratio olorles Final color in 7' _-~_ ~-- olorlessolorlessColorlessYellow , Example 11 To each of the 5 scintillation vials, glutaraldehyde and sodium cyanide were added and mixed first, and lysine solution was added last (Table 10). A yellow color developed from Vial 2 to Vial 5 but not recognizable from Vial 1. A POI was identified between Vial 1 and Vial 3. It is only practical with the naked eye to differentiate the colors between Vial I and Vial 3. That is, it would be challenging to distinguish the difference between Vial 1 and Vial 2 or between Vial 2 and Vial 3.
Thus we may conclude that no narrower POI could be identified unless an instrument is employed.
Table 10.
Glutaraldehyde : Sodium Cyanide Mole Ratio ( 1:1 to 2:1 ).
__ _ Via_I Vial 2 Vial Vial _Vi_al I_ 3 4 5 200u1 200p1 200P1 200p1 200y1 NaCN (82mM) (0.0164 (0.0164 (0.0164 (0.0164 (0.0164 _ _ mMole) mMole) mMole) mMole) mMole) 1600yL 1600p.L 1600p.L 1600~L 1600~.L
Glycine (82mM) (0.1312 (0.1312 (0.1312 (0.1312 (0.1312 mMole) mMole) mMole) mMole) mMole) 93.21 149.1 p1 74.5p.1 111.8~ 130.51 Glutaraldehyde (0.0164 (0Ø.05 ~ (0.0164 (0.0328 ~ (0.008:.
(220mM) solution mMolej mMole) mMole) mNtole) mMole) used _ _ Glutaraldehyde:NaCN1;1 1.25:1 1.5:1 1.75:1 2:1 mole ratio ' Time to develo Never 3' 2' ~ 1' 1' color Color in ~8 minutes Very light Colorless yellow Yellow Yellow Yellow The aldehyde solution can be measured and transferred by means known in the art such as by a regular pipet or syringe. In a preferred embodiment, the aldehyde solution can be measured and transferred using a liquid measuring device as described herein which features a gas or vapor permeable, liquid impermeable, membrane.
The use of the liquid measuring device containing the gas or vapor permeable, liquid impermeable membrane of the present disclosure has the advantage that the liquid can be transferred easily using a simple operation with consistent results.
Compound X and Compound Y (Figure 1) may be in one vial or in two separate 1 ~ vials. Thev may be transferred using either a pipet or syringe. The aldehyde may be added to compound X and the resulting mixture added to compound Y, the aldehyde may be added to compounds X and Y together, or the aldehyde and chemical Y can be added to the chemical X consecutively. The measuring and/or transferring of the aldehyde test sample can be conducted with a regular pipet or syringe. The gas or vapor permeable liquid impermeable barner adds many benefits as described previously.
In one embodiment, shown in Figure 6C, the Compound X may be in a first chamber 9. The aldehyde is drawn up through the valve 8 up to the gas or vapor permeable, liquid impermeable barner 1. After a predetermined time, the aldehyde and compound X are transferred to a second chamber 10 through a valve 8 which is either a one-way or an on/off valve, where they react with compound Y. After a pre-determined time, the color in the second chamber is observed and the presence or absence of excess aldehyde in the test sample is determined.
It will be understood by those of skill in the art that numerous and various modifications can be made without departing from the spirit of the present invention.
Therefore, it should be clearly understood that the forms of the present invention are illustrative only and are not intended to limit the scope of the present invention.
_~5_
Claims (26)
1. A liquid measuring device that measures a fixed volume of liquid comprising:
a first barrel having a proximal and distal end; and a gas or vapor permeable but liquid impermeable barrier situated in the barrel between the proximal and distal ends, whereby the liquid can only be filled up to the barrier.
a first barrel having a proximal and distal end; and a gas or vapor permeable but liquid impermeable barrier situated in the barrel between the proximal and distal ends, whereby the liquid can only be filled up to the barrier.
2. The liquid measuring device of claim 1, wherein the volume in the barrel up to the barrier equals said fixed volume.
3. The liquid measuring device of claim 1, further comprising a means to position said barrier to deliver a fixed volume of liquid, whereby the liquid can only be filled up to the barrier.
4. The liquid measuring device of claim 3, which further comprises a coupling device to adapt the barrier to the measuring device.
5. The liquid measuring device of claim 4, wherein the coupling device comprises an insert.
6. The liquid measuring device of claim 5, wherein the insert is movable in the barrel.
7. The liquid measuring device of claim 5, further comprising a holder to position and secure said insert in the liquid measuring device.
8. The liquid measuring device of claim 6, wherein the insert is moved to a desired position by means of a screw.
9. The liquid measuring device of claim 1 which is a pipette.
10. The liquid measuring device of claim 1 which is a syringe.
11. The liquid measuring device of claim 1, which further comprises a second barrel which is in fluid communication with said first barrel by means of a valve.
12. The liquid measuring device of claim 11 wherein, the valve is a one-way valve.
13. The liquid measuring device of claim 11, wherein the valve has an on/off switch.
14. The liquid measuring device of claim 1, further comprising a needle at the distal end.
15. The liquid measuring device of claim 5, wherein said insert is H-shaped in cross-sectional view.
16. The liquid measuring device of claim 5, wherein said insert is U-shaped in cross-sectional view.
17. The liquid measuring device of claim 1 further comprising a valve at the distal end.
18. The liquid measuring device of claim 17, wherein said valve is a one-way valve.
19. The liquid measuring device of claim 17, wherein said valve is an on/off valve.
20. The liquid measuring device of claim 1, wherein said gas or vapor permeable but liquid impermeable barrier comprises hydrophobic material.
21. A method of measuring a fixed volume of liquid comprising:
providing a gas or vapor permeable but liquid impermeable barrier in a barrel having a proximal end and a distal end;
inserting the distal end into a sample comprising liquid fluid;
creating a negative pressure on the proximal end; and transferring the liquid fluid from the sample into the barrel, wherein the liquid fluid can only be filled up to the barrier.
providing a gas or vapor permeable but liquid impermeable barrier in a barrel having a proximal end and a distal end;
inserting the distal end into a sample comprising liquid fluid;
creating a negative pressure on the proximal end; and transferring the liquid fluid from the sample into the barrel, wherein the liquid fluid can only be filled up to the barrier.
22. The method of claim 21 further comprising adjusting the position of the barrier in the barrel.
23. The method of claim 2l, wherein the barrier is part of a coupling device and the method further comprises adapting the coupling device to the barrel.
24. The method of claim 23, wherein said adapting comprises inserting the coupling device into the barrel.
25. The method of claim 21, wherein the barrel further comprises a valve at the distal end and the method further comprises opening and/or closing the valve.
26. The method of claim 21 further comprising pulling a plunger in the barrier to create a negative pressure.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US09/810,875 | 2001-03-16 | ||
| US09/810,875 US6360595B1 (en) | 2001-03-16 | 2001-03-16 | Liquid measuring device and method of using |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2371975A1 true CA2371975A1 (en) | 2002-09-16 |
Family
ID=25204932
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002371975A Abandoned CA2371975A1 (en) | 2001-03-16 | 2002-02-14 | Liquid measuring device and method of using |
Country Status (7)
| Country | Link |
|---|---|
| US (5) | US6360595B1 (en) |
| EP (1) | EP1241463A3 (en) |
| JP (1) | JP2002357512A (en) |
| KR (1) | KR20020074069A (en) |
| AU (2) | AU785339C (en) |
| CA (1) | CA2371975A1 (en) |
| TW (1) | TW550378B (en) |
Families Citing this family (13)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US6360595B1 (en) * | 2001-03-16 | 2002-03-26 | Ethicon Endo-Surgery, Inc. | Liquid measuring device and method of using |
| SE0102922D0 (en) * | 2001-08-31 | 2001-08-31 | Astrazeneca Ab | Method and apparatus for sample preparation |
| GB0415827D0 (en) * | 2004-07-15 | 2004-08-18 | Univ Manchester | Liquid sampling |
| US7988935B2 (en) * | 2004-09-09 | 2011-08-02 | Microfluidic Systems, Inc. | Handheld and portable microfluidic device to automatically prepare nucleic acids for analysis |
| US8053214B2 (en) * | 2004-09-09 | 2011-11-08 | Microfluidic Systems, Inc. | Apparatus and method of extracting and optically analyzing an analyte from a fluid-based sample |
| US20090177116A1 (en) * | 2006-04-19 | 2009-07-09 | Body Fluid Sampling Device Fluid Measuring Device Using The Same | Body fluid sampling device and body fluid measuring device using the same |
| KR100870875B1 (en) * | 2006-12-29 | 2008-11-28 | 삼성중공업 주식회사 | Test method for soundness of secondary barrier in the liquefied gas tank |
| EP2374541A1 (en) * | 2010-04-06 | 2011-10-12 | Symbion Medical Systems Sàrl | Disposable dispensing cartridge for medical assay instrumentation |
| US20210121884A1 (en) * | 2012-12-21 | 2021-04-29 | Leica Biosystems Melbourne Pty Ltd | Method of producing a reagent on-board an instrument |
| CN103644950B (en) * | 2013-11-15 | 2016-02-24 | 浙江大学 | A kind of fluid experiment waterpower quantitative aerator |
| CN105910673B (en) * | 2016-05-02 | 2019-01-29 | 江苏馨安门窗有限公司 | A kind of integral type solution preparation measurement glass device |
| CN105953862B (en) * | 2016-05-02 | 2018-11-16 | 曹红兵 | A kind of integral type solution preparation measurement glass device |
| CN108827712B (en) * | 2018-07-30 | 2020-12-15 | 六安科科达尔生物科技有限公司 | Waste water collecting, connecting and fixing device and method for wine brewing waste water sampling |
Family Cites Families (40)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US3965032A (en) * | 1973-04-16 | 1976-06-22 | The Dow Chemical Company | Colloidally stable dispersions |
| US3921460A (en) * | 1974-09-06 | 1975-11-25 | Albertus E Schmidlin | Precision liquid-handling instrument |
| US3921480A (en) | 1974-09-12 | 1975-11-25 | Rohr Industries Inc | Form generator for cellular materials |
| US3985032A (en) * | 1975-11-13 | 1976-10-12 | Centaur Chemical Co. | Micropipette filter tips |
| US4059020A (en) * | 1976-09-09 | 1977-11-22 | Centaur Chemical Co. | Filter for micropipettes |
| US4267729A (en) * | 1979-05-14 | 1981-05-19 | Eddelman Roy T | Volumetric pipettor |
| US4327745A (en) * | 1980-09-02 | 1982-05-04 | The Deseret Company | Blood sampling device |
| CA1218930A (en) * | 1984-02-22 | 1987-03-10 | Allelix Biopharmaceuticals Inc. | Device for performing quantitative chemical and immunochemical assays |
| US4889692A (en) * | 1984-11-05 | 1989-12-26 | Holtzman Marc E | Disposable sample preparation container |
| US4601212A (en) * | 1985-07-26 | 1986-07-22 | Shapiro Justin J | Precision micropipettor |
| US4871662A (en) * | 1986-08-11 | 1989-10-03 | Watertest Corporation | Device for shipping microbiology test samples |
| JPS6347665A (en) * | 1986-08-14 | 1988-02-29 | コントロン インスツルメンツ ホールディング エヌ.ブイ. | Method and device for operating pipet |
| DE3635598A1 (en) * | 1986-10-20 | 1988-05-05 | Eppendorf Geraetebau Netheler | PIPETTING DEVICE WITH A CLIP-ON CONE FOR A PIPETTE TIP AND PIPETTE TIP FOR SUCH A PIPETTING DEVICE |
| US4750373A (en) * | 1987-01-22 | 1988-06-14 | Shapiro Justin J | Adjustable volume, pressure-generating pipette sampler |
| US4794806A (en) * | 1987-02-13 | 1989-01-03 | Nicoli David F | Automatic dilution system |
| DE3719302C1 (en) * | 1987-06-10 | 1988-12-29 | Hoyer Gmbh & Co | Device for examining urine |
| DE3722563A1 (en) * | 1987-07-08 | 1989-01-19 | Andreas Szabados | FILTRATION UNIT WITH PRESSURE COMPENSATION |
| AU626796B2 (en) * | 1987-07-13 | 1992-08-13 | City Of Hope | Protein or peptide sequencing method and apparatus |
| DE3807704C1 (en) * | 1988-03-09 | 1989-01-26 | Eppendorf Geraetebau Netheler + Hinz Gmbh, 2000 Hamburg, De | |
| US4936315A (en) * | 1988-10-20 | 1990-06-26 | Lineback Paul I | Methods and apparatus for obtaining arterial blood samples |
| JPH03134997A (en) * | 1989-10-20 | 1991-06-07 | Iwasaki Electric Co Ltd | Metal vapor discharge lamp |
| US5082150A (en) * | 1990-05-01 | 1992-01-21 | Steiner Company, Inc. | Liquid dispensing system including a discharge assembly providing a positive air flow condition |
| US5171537A (en) * | 1991-05-06 | 1992-12-15 | Richard E. MacDonald | Activated immunodiagnostic pipette tips |
| JP3152727B2 (en) * | 1992-03-31 | 2001-04-03 | 株式会社東芝 | Nozzle type analyzer |
| US5360595A (en) * | 1993-08-19 | 1994-11-01 | Miles Inc. | Preparation of diagnostic test strips containing tetrazolium salt indicators |
| US5496523A (en) * | 1994-05-06 | 1996-03-05 | Sorenson Bioscience | Filtered micropipette tip for high/low volume pipettors |
| JPH07306195A (en) * | 1994-05-13 | 1995-11-21 | Ebara Jitsugyo Kk | Method and apparatus for measuring concentration of oxidant component in sea water |
| US5476526A (en) * | 1994-05-13 | 1995-12-19 | Newtron Products Company | Adjustable filter frame and grid |
| US5603900A (en) * | 1995-05-19 | 1997-02-18 | Millipore Investment Holdings Limited | Vacuum filter device |
| US5714696A (en) * | 1995-07-06 | 1998-02-03 | The Regents Of The University Of California | Fluid sampling apparatus and method |
| JPH09196911A (en) * | 1996-01-19 | 1997-07-31 | Fuji Photo Film Co Ltd | Blood filter unit |
| GB9604292D0 (en) * | 1996-02-29 | 1996-05-01 | Hybaid Ltd | Estimation of a nucleic acid |
| US6117394A (en) * | 1996-04-10 | 2000-09-12 | Smith; James C. | Membrane filtered pipette tip |
| US5916524A (en) * | 1997-07-23 | 1999-06-29 | Bio-Dot, Inc. | Dispensing apparatus having improved dynamic range |
| US6045757A (en) * | 1997-06-30 | 2000-04-04 | Rainin Instrument Co., Inc. | Membrane filter pipette tip |
| JP3929571B2 (en) * | 1997-10-15 | 2007-06-13 | パイロットインキ株式会社 | Writing instrument |
| US6387710B1 (en) * | 1998-11-04 | 2002-05-14 | Sarnoff Corporation | Automated sample processor |
| US6368872B1 (en) * | 1999-10-22 | 2002-04-09 | Tecan Trading Ag | Apparatus and method for chemical processing |
| KR100382315B1 (en) * | 2000-07-13 | 2003-05-01 | 유일정공 주식회사 | The DO Sensor Inserted The Spacer |
| US6360595B1 (en) * | 2001-03-16 | 2002-03-26 | Ethicon Endo-Surgery, Inc. | Liquid measuring device and method of using |
-
2001
- 2001-03-16 US US09/810,875 patent/US6360595B1/en not_active Expired - Fee Related
-
2002
- 2002-01-09 US US10/042,906 patent/US6629468B2/en not_active Expired - Fee Related
- 2002-01-09 US US10/042,904 patent/US20020192114A1/en not_active Abandoned
- 2002-02-13 EP EP02250971A patent/EP1241463A3/en not_active Withdrawn
- 2002-02-14 CA CA002371975A patent/CA2371975A1/en not_active Abandoned
- 2002-02-19 TW TW091102729A patent/TW550378B/en not_active IP Right Cessation
- 2002-02-19 AU AU15675/02A patent/AU785339C/en not_active Ceased
- 2002-02-27 KR KR1020020010485A patent/KR20020074069A/en not_active Application Discontinuation
- 2002-03-15 JP JP2002072859A patent/JP2002357512A/en active Pending
-
2003
- 2003-05-30 US US10/448,554 patent/US7073401B2/en not_active Expired - Fee Related
-
2006
- 2006-03-30 US US11/394,049 patent/US7475608B2/en not_active Expired - Fee Related
-
2007
- 2007-02-01 AU AU2007200440A patent/AU2007200440A1/en not_active Withdrawn
Also Published As
| Publication number | Publication date |
|---|---|
| JP2002357512A (en) | 2002-12-13 |
| KR20020074069A (en) | 2002-09-28 |
| US7073401B2 (en) | 2006-07-11 |
| US20030209082A1 (en) | 2003-11-13 |
| US20060243044A1 (en) | 2006-11-02 |
| AU1567502A (en) | 2002-09-19 |
| AU2007200440A1 (en) | 2007-02-22 |
| AU785339C (en) | 2007-10-04 |
| US20020192114A1 (en) | 2002-12-19 |
| US6629468B2 (en) | 2003-10-07 |
| EP1241463A2 (en) | 2002-09-18 |
| US20030037625A1 (en) | 2003-02-27 |
| EP1241463A3 (en) | 2004-02-04 |
| TW550378B (en) | 2003-09-01 |
| US7475608B2 (en) | 2009-01-13 |
| AU785339B2 (en) | 2007-01-18 |
| US6360595B1 (en) | 2002-03-26 |
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| US7475608B2 (en) | Liquid measuring device | |
| US20070086924A1 (en) | Pipette with contamination indicator | |
| CA2427083A1 (en) | Devices and methods for analyte concentration determination | |
| RU2002116402A (en) | Testing device, testing strip, device and method for measuring concentration | |
| EP2140275B1 (en) | Piezo dispensing of a diagnostic liquid into microfluidic devices | |
| EP1500930A1 (en) | Method of measuring formaldehyde concentration of gas and measuring instrument | |
| US8307697B2 (en) | Method for estimating viscosity | |
| EP1256799A2 (en) | Method and apparatus for rapidly assaying aldehyde-containing disinfectant | |
| AU2019336336A1 (en) | Systems, sensors and methods for determining a concentration of an analyte | |
| EP1248104A2 (en) | MBTH for aliphatic aldehyde measurement | |
| AU2006236077A1 (en) | Method and apparatus for rapidly assaying aldehyde-containing disinfectant | |
| US3682586A (en) | Process for the determination of creatinine body fluids | |
| AU2007200682A1 (en) | Liquid measuring device and method of using | |
| CN112469998A (en) | Fluid channel containing conductivity sensor and method of use thereof | |
| AU2006236076A1 (en) | MBTH for aliphatic aldehyde measurement | |
| US20120052588A1 (en) | Means and method for the determination of the aldehyde content | |
| Amelin et al. | Cellulose paper with chemically immobilized 1-naphthylamine for the rapid determination of nitrites, nitrates, and aromatic amines | |
| 조영범 | New paper based ammonia and pH sensors utilizing controlled sample transport and efficient colorimetric detection | |
| US20220362766A1 (en) | Microfluidic Sensor for Continuous or Semi-Continuous Monitoring of Quality of an Aqueous Solution | |
| de la Peña et al. | Simultaneous kinetic-photometric determination of imipramine and desipramine by stopped-flow mixing technique | |
| Crompton et al. | On-Site Measurement of Anions | |
| EP0597900A1 (en) | Colorimetric determination of magnesium ions in fluids |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| EEER | Examination request | ||
| FZDE | Dead |