AU723190B2 - Improved sample card - Google Patents
Improved sample card Download PDFInfo
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- AU723190B2 AU723190B2 AU71911/98A AU7191198A AU723190B2 AU 723190 B2 AU723190 B2 AU 723190B2 AU 71911/98 A AU71911/98 A AU 71911/98A AU 7191198 A AU7191198 A AU 7191198A AU 723190 B2 AU723190 B2 AU 723190B2
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- card
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- Apparatus Associated With Microorganisms And Enzymes (AREA)
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Description
Lj S F Ref: 337645D3
AUSTRALIA
PATENTS ACT 1990 COMPLETE SPECIFICATION FOR A STANDARD PATENT
ORIGINAL
9 *9 Name and Address of Applicant: bioMerleux Vitek, Inc.
595 Anglum Drive Hazelwood Missouri 63042 UNITED STATES OF AMERICA Raymond E. O'Bear, Bruno John Staples Actual Inventor(s): Colin, Garry R. Tegeler and Address for Service: Invention Title: Spruson Ferguson, Patent Attorneys Level 33 St Martins Tower, 31 Market Street Sydney, New South Wales, 2000, Australia Improved Sample Card The following statement is a full description of this invention, including the best method of performing it known to me/us:- 5845 Improved Sample Card Field of the Invention The invention relates to an improved sample card for analysing biological or other samples.
Background of the Invention Biocards have been used to analyse blood or other biological samples in a spectroscopic or other automated reading machine. Such machines receive a small biocard, roughly the size of a playing card, in which biological reagents, nutrients or other material is deposited and sealed, prior to injection of patient samples.
The biocard contains the reagents and receives the patient samples in a series of small wells, formed in the card in rows and columns and sealed, typically with tape on both sides. The biocards are filled with patient sample material through fine hydraulic channels formed in the card. The microorganisms in the samples may then be permitted to grow or reactions to proceed, generally over a period of up to a few hours, although the period varies with the type of bacteria or other substance analysed and sample used.
After the incubation, the samples contained in the wells are placed in front of a laser, fluorescent light or other illumination source. The content of the sample in a given well can then be deduced according to readings on the spectrum, intensity or other characteristics of the transmitted or reflected radiation, since the culture of different bacteria or other agents leave distinctive signatures S:o: related to turbidity, density, byproducts, colouration, fluorescence and so forth. Biocards and 20 machines for reading them of this general type for use in these biochemical applications can for example be seen in US 4 318 994; 4 118 280; 4116 775; 4 038 151; 4 018 652; and 3 957 583.
Despite the general success of biocards in this area, there is an ongoing desire to improve the performance of the cards and readings on their samples. It is for example an advantage to impress more reaction wells in a given card, so that a greater variety of reactions and therefore discrimination 25 of samples can be realised. A given facility may have only one such machine, or be pressed for continuous analysis of samples of many patients, as at a large hospital. Conducting as many identifying reactions on each sample as possible is frequently desirable, yielding greater overall throughput However, biocards that have been exploited commercially have often been limited to a total of 30 sample wells (or 45 wells in some designs). For compatibility with existing reading machines, the cards generally can not be enlarged from a certain standard profile (roughly 88mm by 57mm). Total well capacity has accordingly not grown beyond these levels, limiting the throughput on the machines.
It has also been the case that as the total number of reaction wells on a given card has increased, while the card size has remained constant, the wells have necessarily been formed increasingly close together. With the sample wells crowding each other on the card, it has become more likely that the sample contained in one well can travel to the next well, to contaminate the second well. The threat of increased contamination comes into play especially as card well capacity increases above 30 wells.
2 Summary of the Invention It is accordingly an object of the invention to provide a biocard having an increased number of sample wells.
It is another object of the invention to provide a biocard with increased capacity, yet retaining overall standard card sizes.
It is another object of the invention to provide a biocard which can be loaded with samples quickly, easily and with a minimum of sample corruption.
It is another object of the invention to provide a biocard with improved disposal of injection bubbles arising during loading of the samples.
n It is another object of the invention to provide a biocard which increase the effective fluid flow distance between adjacent wells, reducing well-to-well contamination.
It is another object of the invention to provide a biocard with better, smoother, more reliable fluid flow throughout the card.
The invention achieving these and other objects is an improved biocard having a significantly s improved sample well capacity, easily achieving 45 wells, and reaching 64 wells and feasibly more.
The biocard of the invention likewise provides carefully structured fluid channels which improve fluid flow, reduce bubbling yet improve disposal of any bubbles which do form through specially designed bubble traps.
The biocard of the invention provides, as well, improved security against well-to-well 2 o contamination, in part by increasing the effective distance that the samples in adjacent sample wells S"must travel to corrupt neighbouring sites.
Disclosure of the Invention According to a first aspect of the present invention, there is provided a test sample card comprising: a card body defining a top surface and a bottom surface, a fluid intake port and a plurality of sample wells placed between said first and second end regions and said first and second side regions, a fluid channel network comprising a first distribution channel in communication with said fluid intake port and a second distribution channel connecting said first distribution channel with at least two of said plurality of sample wells, said first and second distribution channels having different crosssectional areas, thereby inhibiting potential cross-contamination between said wells.
o According to a second aspect of the present invention, there is provided A test sample card comprising: a card body defining a first surface and a second surface, a fluid intake port and at a plurality of sample wells placed between said first and second end regions and said first and second side regions, a fluid channel network comprising a first distribution channel in communication with said fluid intake port and a second distribution channel connecting said first distribution channel with at S{awo of said plurality of sample wells, said first and second fluid channels provided in said first
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2a surface of said card; said fluid channel network further comprising a third distribution fluid channel in communication with said fluid intake port, a fourth distribution channel connected to said third fluid channel, and a through-card fluid channel connected to said fourth fluid channel and linking said fourth fluid channel with one of said plurality of sample wells, said third and fourth fluid channels provided in said second surface of said card, whereby said first and second fluid channels in said first surface of said card and said third and fourth fluid channels in said second surface of said card increase the separation distance between said wells of said card, reducing the risk of contamination between said wells.
Brief Description of the Drawings S The invention will be described with reference to the drawings, in which like parts are labelled with like numbers. The drawings are briefly described below.
Figure 1 illustrates an improved biocard according to the invention, in a front planar view.
Figure 2 illustrates the improved biocard according to the invention, in a back planar view.
Figure 3 illustrates the improved biocard according to the invention, in a top edge view.
Figure 4 illustrates the improved biocard according to the invention, in a bottom edge view.
Figure 5 illustrates the improved biocard according to the invention, in a side edge view.
Figure 6 illustrates the improved biocard according to the invention, in an opposite side edge view.
Figure 7 illustrates a sample well with associated fill channel and bubble trap, according to the improved biocard to the invention.
Detailed Description of the Drawings A preferred embodiment of the invention is illustrated in Figures 1-7. This embodiment provides an improved biocard 100, having a generally rectangular shape and in standard dimensions. Biocard o 100 in the illustrated embodiment contains a total of 64 separate sample wells 110, each of which S receives a sample, for example a biological sample extracted from blood, other fluids, tissue or o•S 'Soo Soo other material of a patient, for spectroscopic or other automated analysis. The biological sample may be a direct sample from the patient, or be patient sample which is extracted, diluted, suspended, or otherwise treated, in solution or otherwise. Other types of samples, including antibiotic dosages or other material, can also be introduced for analysis. It will be understood that well capacities other than 64 can be used. Biocard 100 is generally used in a landscape orientation.
In terms of materials, biocard 100 may be made of polystyrene, PET, or any other suitable plastic or other material. Biocard 100 may be tempered during manufacture with a softening material, so that crystalline rigidity, and resultant tendency to crack or chip, is reduced. Biocard 100 for instance may be manufactured out of a blend of polystyrene, approximately 90% or more, along with an additive of butyl rubber to render the card slightly more flexible and resistant to damage. Biocard 100 may also be doped with coloring agents, for instance titanium oxide to produce a white colour, when desired.
The biocard 100 of the invention may be of use in identifying and/or enumerating any number of microorganisms, such as bacterial and/or other biological agents. Many bacteria lend themselves oe•* 15 to automated spectroscopic, fluorescent and similar analysis after incubation, as is known in the art The transmission and absorption of light is affected by the turbidity, density and colorimetric properties of the sample. Fluorescent reactions may be performed as well, independently or along o with spectroscopic or other measurements. If fluorescent data are gathered, use of a coloring agent o in biocard 100 is preferable, since an opaque card reduces or eliminates the scattering of fluorescent 2o emissions throughout the card, as can occur with a translucent material. Other types of detection and analysis can be done on biocard 100, including testing of susceptibility of microorganisms to antibiotics of different types, and at different concentrations, so that biocard 100 is a general-purpose instrument.
To receive sample fluid, the biocard 100 includes a sample intake plenum or port 120 at an upper right corner of the card 100, located on a perimeter edge of the card. The sample wells of card 100 contain dry biological reagents which are previously put in place in the wells, by evaporative, freeze-drying or other means, prior to being dissolved in solution with the injected patient sample for analysis. Each well can hold a deposit of a different reagent, for identifying different biological agents, if desired.
Intake port 120 receives a fluid injection tip and related assembly (schematically illustrated as 130), through which the sample fluid or other solution which arrives to dissolve the biological reagent is injected, under a vacuum pulled on biocard 100 (typically 4.8 to 6.2kPa), then released to atmospheric pressure. Injection port 120 includes a small intake reservoir 140 formed as a roughly rectangular hole through the card 100, which receives incoming fluid, and acts as a fluid buffer.
The fluid (patient sample or other solution) enters intake port 120, collects in intake reservoir 140 and travels along first distribution channel 150, located on the front or facing side of card 100.
First distribution channel 150 consists of a relatively long channel formed in the surface of card 100, which extends substantially across the width of the card, and may have a cross section of approximately mm 2 First distribution channel 150 is tapped at intervals along its length by a series of parallel distribution legs or fill channels 160, which generally descend from channel 150 toward the sample wells 1 10 in each of the eight illustrated columns. When the sample is injected into the card, a short segment of the sample tip can be pinched off or heat sealed and left in place in intake port 120, acting as a sealing plug.
Fill channels 160 are relatively short channels (which may be kinked) which extend down from first distribution channel 140 into respective sample wells 110 located in the first row of card 100, and having a cross section of approximately 0.1-0.2mm 2 It will be appreciated that each of fill channels 160 descend to and enter sample wells 110 at an angle, which results in the natural flow of the sample fluid down through the fill channels 160 by gravity, and resistance to small pieces of undissolved material flowing back up into the fluid circuitry.
When the sample fluid actually enters the well 110, the fluid fills the well by action of both gravity and a vortex-type of flow effect into that well. Also, any of the fill channels 160, as schematically illustrated in Figure 7, as well as other connecting fluid channels in the invention may be preferably formed in full-radius style, that is, as a semicircular conduit rather than a squared-off channel as in some older designs. The full-radius feature has been found by the inventors to reduce friction and fluid o 15 turbulence, further enhancing the performance of biocard 100.
Each of sample wells 110 in the first and other rows includes an associated bubble trap 170, connected to sample well 110 at an upper corner of the well, and located at a height slightly above the well on the card surface. As illustrated in Figure 7, each bubble trap 170 is connected to its respective well by a short trap connecting conduit 180, formed as a hollow passage part-way into the card surface and forming a short conducting path for trapped gaseous bubbles which have been formed in, or communicated to, the well 110 during the injection operation, by bacterial or other S•biological reaction, or otherwise. Bubble trap 170 does not cut through the card completely, instead consisting of a depression or well of roughly cylindrical shape, with a rounded bottom contour, and a volume of approximately 4.2mm 3 in the illustrated embodiment.
Because the bubble trap 170 is located at an elevated position above each respective well 110, any gaseous bubbles will tend to rise and be trapped in the depression of trap 170. With gaseous remnants led off to the bubble trap 170, analytical readings on the biological sample can be made more reliably, since scattering and other corruption of the microbial radiation reading by gas is reduced or eliminated.
As will also be understood from the following, the two-sided nature of biocard 100 permits fluid channels to be formed opposite to non-penetrating bubble traps 170, on the other side of the card.
Some older card designs have employed bubble traps which penetrate through the card, eliminating the possibility of surface channels being routed in their vicinity.
In addition to the introduction of fluid through the path of first distribution channel 150, fluid also travels to wells below the first row of wells through other directions. More specifically, intake port 120 also connects to a second distribution channel 190 formed on the opposite or back surface of the biocard 100, second distribution channel 190 also leading away from the intake reservoir 140.
Second distribution channel 190 also extends substantially along the width of card 100, but on the rear surface of the card. Second distribution channel 190 has a cross-sectional area of approximately 0.2-0.3mm2.
Second distribution channel 190 is tapped above each of the eight illustrated columns of sample wells by a triplet of additional distribution legs or channels 200. Each of triplet legs 200 contains three relatively short connecting channels leading down from second distribution channel to a set of three respective through-channels 210 formed through the body of card 100.
Through-channels 210 are small apertures, approximately 1 mm in diameter, formed cleanly through the body of biocard 100, forming conduits or vias from one surface of the card to the other.
The channels of triplet legs 200 connect to the respective through-channels 210, which in turn are connected to additional well fill channels 220, forming a short link to three additional respective samples wells 110.
However, the fill channels 220 deliver the fluid to the sample wells from the opposite, that is rear, side of the card 100, creating a different fluid flow circuit which extends from intake port 120.
That is, this path involves the second distribution channel on the rear surface of the card, through the body of the card by way of through-channels 210, then out to connecting fill channels 220 which deliver the sample to the well 110 (again at an inclined angle, providing gravity resistance to debris ooooo uptake).
The sample wells which receive the fluid from the second distribution through-channel circuit, like the sample wells which receive the fluid through the (front-planar) first distribution channel, also •have bubble traps 170 associated with them, in the same general above-well configuration.
The biocard 100 therefore includes four rows by eight columns of sample wells built up by connecting channels through the first and second distribution channels. This provides a set of 32 sample wells. In addition, another contiguous set of samples wells, making up the remaining 32 wells for the total of 64, is also deployed along the bottom of the card body using through-channels.
More specifically, a third distribution channel 230 is in fluid connection with intake port 120, but traces a generally vertical path downward from the port to a third distribution through channel 240, located at a lower right section of the card 100. Third distribution channel 230 and its corresponding third distribution through-channel 240 have slightly larger cross sections than the first two distribution channels and their through-channels 210, to accommodate larger fluid flow to a greater total number of destination wells (32, versus 8 and 24 wells, respectively).
The fluid flows down through the third distribution channel 230, into third distribution throughchannel 240, and then splits into two subchannels. The first subchannel 250 on third distribution channel 230, located on the rear of card 100, is a widthwise channel extending along the lower base of the card, having a cross-section of approximately 0.2-0.3mm 2 Rising up from first subchannel 250 are another set of triplet legs 260, which generally resemble first triplet 200 but which extend upward from first subchannel 230, rather than downward.
However, triplet legs 260 perform the same basic function, delivering the fluid to another set of through-channels 270, identical to through-channels 210. Through-channels 270 in turn lead through the card body, that is, to the front of the card, to connecting fill channels 280, which arc generally short concave links (which may be kinked) to respective additional sample wells 110. Fill channels 280 likewise enter the sample wells 110 at an inclined angle, from above.
The last fluid flow path is second subchannel 290, leading off of third distribution throughchannel 240 along the front of card 100, in a generally horizontal or widthwise manner. Second subchannel 290 is connected to the last (eighth), bottom row of eighth sample wells 110 by another set of vertical connecting conduits 300, single conduits connecting to single wells. Conduits 300 are generally dog-legged in structure, enter the well at a slightly inclined angle, and the associated wells each also include an associated bubble trap 170.
It may thus be seen that through the use of through-channels penetrating the card body 110, along with carefully distributed links through a plurality of distribution channels, in the invention valuable surface area is freed up on the card, by allowing the necessary connecting channels to be split up between the front and rear surfaces of the card.
The fluid flow paths thoroughly dispersed over card 100, including both front and rear surfaces, also result in a longer total linear travel of the flowing fluid than conventional cards. This leads to the significant advantage that the possibility of inter-well contamination is reduced. The well-to-well distance in fact in the illustrated embodiment comes to approximately 35mm, significantly more than the 12mm or so on many older card designs.
The inventors have also observed that the rate of inter-well contamination varies with the square of the linear distance, so the elongated fluid paths significantly enhance the integrity of readings on the card. Contamination itself is a function of sample mixing (density of solution falling oooout of wells) and liquid molecular diffusion, both of which are discouraged by the relatively fine channel cross-sections in many sections of the Overall fluid circuit, as well as overall path length.
The contamination rate is also reduced by the fact that the volume of the channels along the S"fluid circuit varies slightly along the overall circuit travelled by a given sample. That is, the throughchannels, the three main distribution channels and other segments of the paths have cross-sectional areas which, although all relatively fine, may differ slightly. The change in volume over the path tends a to retard the progression of contamination, as do dog-legged or kinked sections of connecting conduits.
All these structural adaptations cooperate in reducing the rate of inter-well contamination in the biocard 100. The inventors have, as one indication of contamination management, measured the time required for test dye to infiltrate a neighbouring well in conventional biocards and the card of the invention. Contamination in a conventional, low-capacity, non-through-body card has been observed in approximately 24 hours. In the biocard of the invention under similar conditions, in contrast, the contamination time has been observed at 16-18 hours.
Besides contamination kinematics, the upper-placed bubble traps 170 also more efficiently scrub the sample wells 110 of gas bubbles which form after the sample injection. Samples are typically injected as noted by evacuating the card, introducing fluid at the intake and then releasing the vacuum pull, so that the whole fluid circuitry returns to atmospheric pressure. Vacuum filling of the card may typically be done over a period of 3-60 seconds, slower rates helping to reduce the tendency of bubbles to form. Those bubbles can ruin sample readings, so reducing them results in a smoother, more efficient, higher-capacity yet more reliable biocard.
In addition, the improved fluid circuitry of biocard 100, including full-radius fill and other channels, generally narrower channels than older card designs, width-variation and other features result in a high capture percentage of sample intake actually reaching the sample wells 110, which the inventors have calculated at as high as 90-95%. This compares with a capture percent in the for older card designs.
For mechanical interaction with the automated reading machine, biocard 100 may also be provided with a series of sensor stop holes 310, located along the bottommost edge of the card.
Sensor stop holes 310, illustrated as regularly spaced, rectangular through-holes, permit associated photodetectors to detect when a biocard 100 mounted in a reading machine has come into proper lo alignment for optical reading. The sensor stop holes 310 are arranged in vertical register with the vertical columns of wells 110, so that the optical detection of the stop hole 310 corresponds exactly to positioning of the sample wells 110 before optical reading devices. Older biocards have been aligned by sensor holes which are formed not integrally with the card itself, but in carriages or other supports which are attached to the card at some point in the reading process, as for instance disclosed in US 4 118 280. These structures have however been prone to time-consuming maintenance, particularly requiring the mechanical calibration and lining up of the carriage with the cards, and photodetectors.
Integral sensor stop holes 310 eliminate that type of difficulty.
The biocard 100 of the invention is formed in the illustrated embodiment, as shown in Figure 7, with a mould parting line 320 which is formed most of the way down into a sample well 110, toward the bottom of the card as opposing mould dies meet during manufacture. Older card designs often had the mould parting line, which forms a tiny lip in a fluid cavity, at an upper point (above midway) of the card. The upper mould parting lines could tend to induce annular bubble rings to form during filling, as well as reduce the efficiency of drying of antibiotics or other material during manufacturing.
The use of a downward offset mould parting line 320 avoids these difficulties, as well as improving the efficiency of chemical or antibiotic dehydration during incubation, and may act as a slight aperture 0 during light and fluorescence reading operations. As illustrated in Figure 7, the walls of the sample oleo well, and other features, are usually formed at a slight angle or incline (typically 140), as an artefact of Sconventional moulding processes in which separating the moulded part from opposing moulding pieces is made easier with slight surface inclinations. The shifting of the mould parting line 320 to the bottom area of biocard 100 likewise results in a smaller inclined (roughly speaking, trapezoidal) area in the bottom of the sample well which can tend to trap material, slightly.
Another advantage of biocard 100 of the invention is that patient sample and other markings are not introduced directly on the card itself, in pre-formed segments, as for example shown in aforementioned US 4 116 775 and others. Those on-card stipplings and markings can contribute to debris, mishandling and other problems. In the invention, instead, the card may be provided with barcoding or other data markings by adhesive media, but markings or pre-formed information segments are not necessary (though some could be imprinted if desired) and debris, mishandling, loss of surface area and other problems can be avoided.
Biocard 100 furthermore includes, at the lower left corner of the card as illustrated in Figure 1, a tapered bezel edge 330. Tapered bezel edge 330 provides an inclined surface for easier insertion of 8 biocard 100 into, carousels or cassettes, into slots or bins for card reading, and other loading points in the processing of the card. Tapered bezel edge 330 provides a gently inclined surface, which relieves the need for tight tolerances during loading operations.
Biocard 100 also includes a lower rail 360 and an upper rail 370, which are slight structural s "bulges" at along the top and bottom areas of the card to reinforce the strength and enhance handling and loading of the biocard 100. The extra width of lower and upper rails 360 and 370 also exceeds the thickness of sealing material, such as adhesive tape, that is affixed to the front and back surfaces of biocard 100 for sealing during manufacture and impregnation with reagents. The raised rails therefore protect that tape, especially edges from peeling, during the making of the biocard 100, as well as during handling of the card, including during reading operations.
Upper rail 370 may have serrations 390 formed along its top edge, to provide greater friction when biocard 100 is transported in card reading machines or otherwise using belt drive mechanisms.
Lower card rail 360 may also have formed in it reduction cavities 380, which are small elongated depressions which reduce the material, weight and expense of the card by carving out space where :ri 15 extra material is not necessary in the reinforcing rail 360.
In terms of sealing of biocard 100 to contain reagents and other material, it has been noted that sealing tapes are typically used to seal flush against biocard 100 from either side, with rail protection.
Biocard 100 also includes a leading lip 340 on lower card rail 360, and on upper card rail 370 which °projects slightly over the leading edge of the card. Conversely, at the opposite end of the biocard 100 there is a trailing truncation 350 in both rails. This structure permits sealing tape to be applied in the card preparation process in a continuous manner, with card after card having tape applied, then the tape cut between successive cards without the tape from successive cards getting stuck together.
The leading lip 340 and trailing truncation 350 provides a clearance to separate cards and their rr' applied tape, which may be cut at the trailing truncation 350 and wrapped back around the card edge, for increased security against interference between abutting cards.
The foregoing description of the improved biocard of the invention is illustrative, and variations on certain aspects of the inventive system will occur to persons skilled in the art. The scope of the invention is accordingly intended to be limited only by the following claims.
Claims (4)
1. A test sample card comprising: a card body defining a top surface and a bottom surface, a fluid intake port and a plurality of sample wells placed between said first and second end regions and said first and second side regions, a fluid channel network comprising a first distribution channel in communication with said fluid intake port and a second distribution channel connecting said first distribution channel with at least two of said plurality of sample wells, said first and second distribution channels having different cross-sectional areas, thereby inhibiting potential cross-contamination between said wells.
2. A test sample card comprising: a card body defining a first surface and a second surface, in, a fluid intake port and at a plurality of sample wells placed between said first and second end regions and said first and second side regions, a fluid channel network comprising a first distribution channel in communication with said fluid intake port and a second distribution channel connecting said first distribution channel with at least two of said plurality of sample wells, said first and second fluid channels provided in said first surface of said card; said fluid channel network further comprising a is third distribution fluid channel in communication with said fluid intake port, a fourth distribution channel connected to said third fluid channel, and a through-card fluid channel connected to said fourth fluid 0 channel and linking said fourth fluid channel with one of said plurality of sample wells, said third and 0 fourth fluid channels provided in said second surface of said card, whereby said first and second fluid channels in said first surface of said card and said third and fourth fluid channels in said second ,o surface of said card increase the separation distance between said wells of said card, reducing the risk of contamination between said wells.
3. The test sample card of claim 2, wherein each of said sample wells comprising a bubble trap connected to said sample wells by a connecting conduit with said connecting conduit formed in said first surface of said card but not in said second surface, said bubble traps comprising depressions in said first surface of said card extending part way through said card, said bubble traps thereby formed in an elevated position with respect to said sample wells.
4. A test sample card as described in claim 2, said card substantially as hereinbefore described with to the accompanying drawings. Dated 16 May, 2000 bioMerieux Vitek, Inc Patent Attorneys for the Applicant/Nominated Person A_ SPRUSON FERGUSON [1:\Day ib\LI BLJU]07277.doc:tlt
Priority Applications (1)
Application Number | Priority Date | Filing Date | Title |
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AU71911/98A AU723190B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
Applications Claiming Priority (3)
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US455534 | 1995-05-31 | ||
AU54591/96A AU695716B2 (en) | 1995-05-31 | 1996-05-29 | Improved sample card |
AU71911/98A AU723190B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
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AU54591/96A Division AU695716B2 (en) | 1995-05-31 | 1996-05-29 | Improved sample card |
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AU7191198A AU7191198A (en) | 1998-10-01 |
AU723190B2 true AU723190B2 (en) | 2000-08-17 |
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AU71912/98A Ceased AU722719B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
AU71910/98A Ceased AU722698B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
AU71913/98A Ceased AU722763B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
AU71911/98A Ceased AU723190B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
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AU71910/98A Ceased AU722698B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
AU71913/98A Ceased AU722763B2 (en) | 1995-05-31 | 1998-06-16 | Improved sample card |
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Publication number | Priority date | Publication date | Assignee | Title |
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US9757723B2 (en) | 2010-10-08 | 2017-09-12 | Biomerieux, Inc. | Sample test cards |
EP2643679A4 (en) | 2010-11-23 | 2017-10-11 | Biomerieux, Inc | Improved sample test cards |
KR101446526B1 (en) * | 2013-05-02 | 2014-10-08 | 주식회사 퀀타매트릭스 | Cell culture analyzing device based on microfluidic multi-well format |
KR101396110B1 (en) | 2013-10-30 | 2014-05-16 | 아주대학교산학협력단 | Aliphatic polycarbonate and its aromatic polyester copolymers having long chain branches |
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US4116775A (en) * | 1976-05-03 | 1978-09-26 | Mcdonnell Douglas Corporation | Machine and process for reading cards containing medical specimens |
US4818493A (en) * | 1985-10-31 | 1989-04-04 | Bio/Data Corporation | Apparatus for receiving a test specimen and reagent |
US5374395A (en) * | 1993-10-14 | 1994-12-20 | Amoco Corporation | Diagnostics instrument |
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US4038151A (en) * | 1976-07-29 | 1977-07-26 | Mcdonnell Douglas Corporation | Card for use in an automated microbial detection system |
US5110727A (en) * | 1987-04-03 | 1992-05-05 | Cardiovascular Diagnostics, Inc. | Method for performing coagulation assays accurately, rapidly and simply, using dry chemical reagents and paramagnetic particles |
DE69330772T2 (en) * | 1992-03-09 | 2002-07-04 | Accumed International Inc., Chicago | DIAGNOSTIC MICROBIOLOGICAL TEST DEVICE AND METHOD |
DE69329424T2 (en) * | 1992-11-06 | 2001-04-19 | Biolog, Inc. | TEST DEVICE FOR LIQUID AND SUSPENSION SAMPLES |
US5342581A (en) * | 1993-04-19 | 1994-08-30 | Sanadi Ashok R | Apparatus for preventing cross-contamination of multi-well test plates |
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1998
- 1998-06-16 AU AU71909/98A patent/AU722123B2/en not_active Ceased
- 1998-06-16 AU AU71912/98A patent/AU722719B2/en not_active Ceased
- 1998-06-16 AU AU71910/98A patent/AU722698B2/en not_active Ceased
- 1998-06-16 AU AU71913/98A patent/AU722763B2/en not_active Ceased
- 1998-06-16 AU AU71911/98A patent/AU723190B2/en not_active Ceased
Patent Citations (3)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US4116775A (en) * | 1976-05-03 | 1978-09-26 | Mcdonnell Douglas Corporation | Machine and process for reading cards containing medical specimens |
US4818493A (en) * | 1985-10-31 | 1989-04-04 | Bio/Data Corporation | Apparatus for receiving a test specimen and reagent |
US5374395A (en) * | 1993-10-14 | 1994-12-20 | Amoco Corporation | Diagnostics instrument |
Also Published As
Publication number | Publication date |
---|---|
AU722123B2 (en) | 2000-07-20 |
AU7191298A (en) | 1998-10-01 |
AU722719B2 (en) | 2000-08-10 |
AU722763B2 (en) | 2000-08-10 |
AU7191098A (en) | 1998-10-01 |
AU7191198A (en) | 1998-10-01 |
AU722698B2 (en) | 2000-08-10 |
AU7191398A (en) | 1998-10-01 |
AU7190998A (en) | 1998-10-01 |
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Legal Events
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FGA | Letters patent sealed or granted (standard patent) |