Patent Grant
7320777
1. Field of the Invention
The present invention relates to apparatus for handling microcards used for performing polymerase chain reactions (PCR), for example, and, more particularly, to a device for positioning such microcards in relation to a PCR instrument.
2. Description of the Related Art
A substrate for simultaneously testing a large number of analytes, which has a small sample size and a large number of detection chambers, has been described in published PCT International Application, WO97/36681, assigned to the assignee of the present application, the contents of which are hereby incorporated by reference herein. Also, in commonly assigned U.S. patent application Ser. No. 09/549,382, filed Apr. 13, 2000, now U.S. Pat. No. 6,272,939, the complete disclosure of which is incorporated by reference, a further development of a card-like substrate member having a plurality of sample detection chambers is disclosed together with a system for filling the member with a liquid sample to react with reagents located in the sample detection chambers during thermal cycling of a PCR process. Such card-like substrate members are a spatial variant of the micro-liter plate and are referred to hereinafter as “microcards.” However, the microcards are often referred to in the art as “consumables” because they are relatively inexpensive and disposable after use, and as such, may be made from a variety of different materials and may assume different shapes and sizes.
Microcards typically contain 96, 384, or more, individual sample chambers, each having a volume of about 1.0 μL or less in a card size of 7 cm×11 cm×0.2 cm, for example. Although both the number of sample chambers and the volume size of the individual sample chambers may vary widely, the relatively small size of the microcards present problems in transporting them into and out of a PCR instrument, such as instrument models 7700 or 7900HT available from Applied Biosystems of Foster City, Calif., and aligning the microcard with a thermal cycling block and an optical system in the PCR instrument.
Handling, including placing and removing microcards into and from thermal cyclers of a PCR instrument, storing, and transporting of the microcards may be accomplished either manually or robotically. A robot typically functions by gripping the sides of the microcard by “fingers”, or grips. Because a microcard may have a relatively thin body, with side edges as thin as 0.5 mm or less in thickness, robotic handling may become impractical or inconsistent, especially when multiple microcards are stacked together. Additionally, to accomplish real time PCR processing the microcard must be aligned with an optical reading device, such as a CCD or laser scanner. To be effective, such alignment requires high precision usually greater than tolerances provided by the edges of the microcard. There is a need for reliable alignment of a microcard with a scanner, camera, or luminometer of a PCR instrument.
In addition to the problems associated with alignment, PCR processing requires uniform and complete contact of the sample chambers of the microcard with a thermal cycling block of a PCR instrument. In some instances, where the microcard is formed by laminated plastic materials, there is a tendency for warpage of the card from an initial planar configuration. Thus, to ensure complete contact of the sample chambers of the microcard with the surface of the thermal cycling block, a flexing of the microcard is required so that is conforms to the typically planar surface of that block. In other instances, the microcard may be formed of flexible material incapable, in itself, to maintain a shape that conforms to the surface of the thermal cycling block. In positioning the latter types of microcards relative to the thermal cycling block of a PCR instrument, therefore, provision must be made to conform the microcard to the surface of the thermal cycling block.
Thus, it will be appreciated that there is a need for improvements in apparatus for positioning microcards of the types mentioned above in relation to a PCR instrument, and to facilitate handling of such microcards in general.
The advantages and purpose of the invention will be set forth in part in the description which follows, and in part will be obvious from the description, or may be learned by practice of the invention. The advantages and purpose of the invention will be realized and attained by means of the elements and combinations particularly pointed out in the appended claims.
To attain the advantages and in accordance with the purpose of the invention, as embodied and broadly described herein, the invention is directed to a device for handling PCR microcards, each having an array of sample chambers closed by a transparent material on one side thereof, in relation to a PCR instrument. The device includes a carrier having an apertured region with an array of holes corresponding in number and relative location with the array of sample chambers in each of the microcards, and a structure for retaining a microcard on the carrier so that the transparent material faces the apertured region with the sample chambers aligned, respectively, with the holes in the apertured region, and so that the side of the microcard opposite the transparent material is unobstructed at least throughout the array of sample chambers. Also structure is provided for positioning the microcard retained on the carrier in relation to the PCR instrument.
In another aspect, the advantages and purpose of the invention are attained by such a device having a carrier plate including the apertured region, and a peripherally closed retention frame having an opening at least as large as the array of sample chambers and being fitted to the carrier to retain the microcard in relation to the carrier plate.
In yet another aspect, the advantages and purpose of the invention are attained by such a device for a microcard that has through-holes in marginal portions thereof outside the array of sample chambers, a plate member including the apertured region, and pins projecting from the plate member outside of the apertured region to engage in the through-holes in the marginal areas of the microcard.
In a further aspect, the advantages and purpose of the invention are attained by a PCR kit including at least one handling device, a supply of microcards, and optionally, the appropriate thermal block for processing the supplied microcard. Other kits might include microcards filled with reagents of a supplier's design or custom reagents ordered by a customer. The appropriate handling device would be included with the filled microcards.
It is to be understood that both the foregoing general description and the following detailed description are exemplary and explanatory only and are not restrictive of the invention, as claimed.
The accompanying drawings, which are incorporated in and constitute a part of this specification, illustrate several exemplary embodiments of the invention and together with the description, serve to explain the principles of the invention. In the drawings,
Reference will now be made in detail to the exemplary embodiments of the invention, examples of which are illustrated in the accompanying drawings. Wherever possible, the same reference numbers will be used throughout the drawings to refer to the same or like parts.
In accordance with the present invention, a device is provided for handling PCR microcards, each having an array of discreet reagent containing sample chambers closed by a transparent material on one side thereof, in relation to a PCR instrument. Each sample chamber preferably contains an analyte-specific reagent that reacts with a selected analyte that may be present in the liquid sample. The device is designed for retaining a micro-card on a carrier so that a transparent side of the microcard faces an apertured region of the carrier with the reagent sample chambers aligned, respectively, with the holes in the apertured region, and so that the opposite side of the microcard is unobstructed at least throughout the array of reagent containing sample chambers. As disclosed herein and shown in
Although the microcard 10 and a system for filling it with sample liquid is fully disclosed in the above cited U.S. patent application Ser. No. 09/549,382, filed Apr. 13, 2000, now U.S. Pat. No. 6,272,939, incorporated herein by reference, the features of the microcard 10 that are applicable to the apparatus of the present invention will be described below.
The microcard 10 is formed by a laminated substrate shown in
As embodied herein and shown in
The top and bottom plates 16 and 18 can be joined to each other by a variety of methods so that the network of passageways may be evacuated by a vacuum source, so that the liquid sample does not leak from the substrate, and to withstand temperature fluctuations that can occur during thermal cycling. Preferably, the plates 16 and 18 are joined using ultrasonic welding, but other suitable methods include the use of adhesives, pressure-sealing, or heat curing.
As embodied herein and shown in
As described fully in the above-cited U.S. application Ser. No. 09/549,382, now U.S. Pat. No. 6,272,939, the attachment/bladder groove 26 provides an air pocket for the liquid sample in the network of passageways so that when the filled substrate undergoes temperature fluctuations during thermal cycling operations expansion of the liquid sample in the network 12 of passageways occurs without significantly increasing the pressure on the substrate. Also, the liquid sample may flow into the attachment/bladder groove 26 through sample port 24 under such conditions.
The top and bottom plates 16 and 18 may be made out of any suitable material that can be manufactured according to the required specifications, can withstand any temperature fluctuations that may later occur, i.e., during thermal cycling or other operations performed on the substrate, and can be suitably joined. In addition, for real time optical detection of liquid samples during thermal cycling, the top of each sample detection chamber 14 must be optically transparent for detection of the reaction. For this purpose, silica-based glasses, quartz, polycarbonate, or any optically transparent plastic layer, for example, may be used. For use in PCR reactions, the material should be PCR compatible, and the material should be preferably be substantially fluorescence free. In one embodiment, the material for the top plate is a polycarbonate manufactured by “BAYER”™, referred to as FCR 2458-1112 and the material for the bottom plate is a 0.015 inch thickness polycarbonate manufactured by “BAYER”™, referred to as Makrofol DE1-1D. The substrate plates can be formed by a variety of methods known in the art. For example, top plate 16 may be injection molded, whereas bottom plate 18 may be die-cut. Any other suitable method of manufacturing the plates is also acceptable.
Prior to assembly of the top and bottom plates 16 and 18, an analyte-specific reagent is typically placed in each detection chamber 14. One or more of the detection chambers may be left empty to function as a control. These analyte-specific reagents in the detection chambers may be adapted to detect a wide variety of analyte classes in the liquid sample, including polynucleotides, polypeptides, polysaccharides, and small molecule analytes, by way of example only. The polynucleotide analytes are detected by any suitable method, such as polymerase chain reaction, ligase chain reaction, oligonucleotide ligation assay, or hybridization assay. A preferred method of polynucleotide detection is the exonuclease assay referred to as “TAQMAN”™. Non-polynucleotide analytes may also be detected by any suitable method, such as antibody/antigen binding. The above detection methods are well-known in the art. They are described in detail in the following articles and patents: U.S. Pat. No. 5,210,015 of Gelfand et al.; U.S. Pat. No. 5,538,848 of Livak et al.; WO 91/17239 of Barany et al. published on Nov. 14, 1991; “A Ligase-Mediated Gene Detection Technique” by Landegren et al published in Science 241:1077–90 (1988); “High-density multiplex detection of nucleic acid sequences: oligonucleotide ligation assay and sequence-coded separation” by Grossman et al., published in Nucleic Acid Research 22:4527–34 (1994); and “Automated DNA diagnostics using an ELISA-based oligonucleotide ligation assay” by Nickerson et al., published in Proc. Natl. Acad. Sci. USA 87:8923–27 (1990).
In
A heated cover plate 42, represented schematically by phantom lines in
In accordance with the present invention, the handling device 30 includes a carrier having an apertured region with an array of holes corresponding in number and relative location with the array of reagent containing sample chambers in each of the micro-cards, means for retaining a micro-card on the carrier so that the transparent material of the microcard faces the apertured region with the reagent sample chambers aligned, respectively, with the holes in the apertured region, and so that the side of the micro-card opposite the transparent material is unobstructed at least throughout the array of reagent containing sample chambers. The handling device 30 additionally includes means for positioning the carrier and the micro-card retained thereon in relation to the PCR instrument.
In the illustrated embodiment, the handling device 30 defines a two-part carrier for the microcard 10, the two parts being a peripherally closed frame-like retention frame 44 and a carrier 46 having an array of holes 48 in a central apertured region, the holes corresponding in number and in location with the sample chambers 14 in the microcard 10.
As may be seen in
To retain the microcard 10 by the retention frame 44, both ends of the microcard 10 overlie a pair of tabs 56 that project from opposite inner edges of the marginal flange 52 of the retention frame 44. Except for those retained end portions that overlie the tabs 56, the entire bottom surface of the microcard 10 is exposed through the opening 54 defined by the inner edges of the marginal flange 52.
The carrier 46 is defined in substantial measure by a flat plate 58, in which the array of holes 48 are formed. A peripheral wall 60, of a depth to project both above and below the plate 58, extends about three sides of the plate 58, as shown in
The peripheral edge surfaces of the carrier 46 are shaped and sized to fit somewhat loosely into the peripheral wall 49 of the retention frame 44. When the carrier 46 and retention frame 44 are assembled about a microcard 10 in a manner to be described below, a pair of clips 68 on each of opposite sides of the carrier 46 engage in apertures 70 on opposite sides of the retention frame 44 to secure the assembly. The clips 68 may be released from the apertures 70 by distorting the retention frame of by inserting a tool, such as a small screw driver, through the apertures and flexing the clips to permit removal of the microcard 10 from the device 30.
In
As shown in
As mentioned above with reference to
The carrier 46 and retention frame 44 are preferably constructed of a polymer that is able to withstand the heat used in a typical thermal cycling process, e.g., about 60° to 100° C. Thus, the handling device 30 should be able to maintain its original shape even after multiple thermal cycling processes. The device 30, described herein by way of example, is intended to be reusable and able to substantially maintain its shape after 50 or more hours of thermal cycling. A shelf life of about 5 years would also be expected. Materials that may be used for construction of the device 30 include polymers, plastics, glass, ceramics, metals, or others known in the art that are able to withstand the thermal cycling process. Furthermore, the handling device 30 of this invention may be manufactured in a variety of ways known in the art, including injection molding, machining, or metal stamping methods.
In
As shown in the vastly enlarged fragmentary cross-section of
As shown in
In accordance with the present invention, a device for handling PCR microcards of the type shown in
In the embodiment illustrated in
To ensure thermal insulation and to provide good contact between the microcard 80 and a thermal cycling block to be described below, the silicone rubber compression pad 104 is situated in the recessed region 116 and to be positioned between the carrier frame 102 and the microcard 80 in use. The compression pad 104 also has three hundred and eighty four holes 122 aligned to the holes 119 in the carrier frame so not to obstruct the sample wells from the optics of the PCR instrument. The compression pad 104 is bonded to the recessed region on the underside of the carrier frame and becomes an inseparable part of the handling device 100.
On the underside of the carrier frame 102 in proximity to where the microcard fill port 84 will be located in use, the recessed region 118 is formed with a semi-circular raised region or ledge 124. The compression pad 104 is provided with a complementary semi-circular tab extension 126 located to be positioned on the ledge 124 when the compression pad 104 is secured in the recessed region 118. A combination of the raised ledge 124 and the tab extension 126 functions to ensure that more pressure is applied to the fill port region when the heated cover of the PCR instrument is lowered. A higher compressive force around the region of the fill port 84 prevents samples from leaking from the microcard via the fill port that is sealed with an adhesive tape (not shown).
To secure the microcard 80 to the underside of the carrier frame 102 and against the compression pad 104, and for positioning and aligning the microcard 80 in the PCR instrument, the pins 106, 108110, and 112 protrude from the bottom of the carrier frame 102 in the outer marginal edges 118. When assembling the microcard 80 to the handling device 100, the pins 106 and 112 are inserted into two similarly positioned holes 92 in the microcard 80. A close press fit between the pins 106 and 112 and the holes 92 ensure proper alignment of the microcard with the card carrier frame 102. The press fit also prevents the microcard from separating from the card carrier during transport and handling. The two other pins 108 and 110 protrude from the underside of the card carrier and these pins, together with the two alignment pins 106 and 112, function as legs and provide a means for stacking multiple handling devices 100 with microcards assembled to them. The pins 108 and 110 also augment retention of the microcard 80 to the bottom of the carrier frame 102.
In
In accordance with the present invention, the microcards 10 and 80 and the respective handling devices 30 and 100 are assembled in PCR processing kits, each such kit including at least one handling device 30, 100 and a supply of microcards 10, 80. A kit for use with PCR instrument model 7900HT sold by Applied Biosystems of Foster City, Calif., for example, would additionally include the appropriate thermal block 38 or 130, depending on whether the kit includes microcards 10 or 80. Other kits might include microcards filled with reagents of a supplier's design or custom reagents ordered by a customer. The appropriate handling device would be included with the filled microcards.
Other embodiments of the invention will be apparent to those skilled in the art from consideration of the specification and practice of the invention disclosed herein. It is intended that the specification and examples be considered as exemplary only, with a true scope and spirit of the invention being indicated by the following claims.
This application is a continuation of application Ser. No. 09/897,500, filed Jul. 3, 2001, now U.S. Pat. No. 6,514,750, which is incorporated herein by reference.
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| Number | Date | Country | |
|---|---|---|---|
| 20030124714 A1 | Jul 2003 | US |
| Number | Date | Country | |
|---|---|---|---|
| Parent | 09897500 | Jul 2001 | US |
| Child | 10301870 | US |
