WO2000033962A1 - Rotary thermocycling apparatus - Google Patents
Rotary thermocycling apparatus Download PDFInfo
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- WO2000033962A1 WO2000033962A1 PCT/CA1999/001035 CA9901035W WO0033962A1 WO 2000033962 A1 WO2000033962 A1 WO 2000033962A1 CA 9901035 W CA9901035 W CA 9901035W WO 0033962 A1 WO0033962 A1 WO 0033962A1
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- station
- sample
- container
- spray
- reaction
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L7/00—Heating or cooling apparatus; Heat insulating devices
- B01L7/52—Heating or cooling apparatus; Heat insulating devices with provision for submitting samples to a predetermined sequence of different temperatures, e.g. for treating nucleic acid samples
Definitions
- the present invention relates to a rotary thermocycling apparatus, and to methods of using rotary thermocycling apparatus, especially for use in biochemical reactions and in particular for use in polymerase chain reactions (PCR).
- the present invention is directed to rotary thermocycling processes in which samples are placed on filters, or other media, and heated on plates in a sequence at predetermined temperatures, preferably including at least one step in which the sample is sprayed e.g. with liquid reagent(s), during each cycle.
- the present invention will be particularly described herein with respect to biochemical reactions. It is frequently necessary or desirable to be able to quantify and/or detect the presence of certain nucleic acid molecules or microorganisms in samples of air, soils, water, food, body fluids and other materials. This may be necessary in relation to an immediate medical or health situation, or in testing to determine safety for use by humans or animals. Thus, in many instances, it is important to be able to accurately and quickly confirm the presence and quantity of, or absence of, particular microorganisms in samples, and to do so in an automated, reliable and reproducible manner.
- nucleic acids either double-stranded deoxyribonucleic acids (DNA) or ribonucleic acid (RNA), and detection and discrimination on the basis of specific nucleic acid sequences has permitted the detection of the presence or absence of a particular organism within a test sample.
- PCR polymerase chain reaction
- thermocyclers used for DNA amplification and sequencing in which one or more temperature controlled elements or "blocks" hold samples containing the reaction mixture, and the temperature of the block is varied over time.
- a robotic arm is used to move mixtures from one block to another.
- PCR Polymerase chain reaction
- an enzyme with polymerase activity catalyzes synthesis of a new polynucleotide strand that incorporates the primer oligonucleotide and uses the original denatured polynucleotide as a synthesis template to produce a new double-stranded polynucleotide molecule.
- This series of steps constitutes a PCR cycle. As cycles are repeated, the amount of newly synthesized polynucleotide increases geometrically because the newly synthesized polynucleotides from an earlier cycle can serve as templates for synthesis in subsequent cycles.
- Primer oligonucleotides are typically selected in pairs that can anneal to opposite strands of a given double-stranded polynucleotide sequence so that the region between the two annealing sites is amplified.
- the temperature of the reaction mixture must be varied during each PCR cycle, and consequently varied many times during a test. For example, denaturation of DNA typically takes place at about 90°-100°C, annealing a primer to the denatured DNA is typically performed at about 40°-60°C., and the step of extending the annealed primers with a thermostable DNA-polymerase is typically performed at about 70°-75°C. Each of these steps may have an optimal temperature.
- US 4,981 ,801 describes an apparatus for carrying out enzymatic cycling reactions including a turntable, a number of reaction vessels arranged in the turntable around the periphery and means to circulate antifreeze liquid through the reaction tank. Heaters and refrigerators are provided in order to obtain variations in temperature.
- An apparatus to detect and enumerate a particulate analyte in a liquid sample comprising a filter element in a holder and means to heat and control the temperature of the filter element, is disclosed in WO 94/21780 of R.G.L. Wheatcroft and W.B. Berndt.
- a method for detection and discrimination of multiple analytes using fluorescent technology is disclosed in US 5,723,294. Additional apparatus and methods for conducting thermocycling reactions, especially polymerase chain reactions, in a rapid automated and controlled manner would be beneficial.
- thermocycling apparatus especially for biochemical reactions, comprising:
- said station of (d) is adapted for removal of a cover plate from said container prior to activation of the spray, and for replacement of the cover plate after said spray has terminated.
- the container is a flat-bottomed container of a dimension less than that of the station.
- the heating is comprised of a section with a flat lower surface that is adapted to be lowered into said container close to but not in contact with the sample in said container, especially into contact with a cover plate therein.
- the apparatus has a programmer for controlling at least (i) the temperature at each station, (ii) the dwell time in each station, (iii) the duration and timing of the spray, (iv) the number of sequential cycles for the biochemical reaction.
- the container is adapted to receive a filter having the sample thereon, and to receive a cover plate over said filter.
- the apparatus is programmable and automated.
- the apparatus is adapted to process more than one sample at a time, up to one for each station in the apparatus.
- the heating units are on pistons that are lowered into the containers.
- Another aspect of the present invention provides a method for a sequential reaction, especially a sequential biochemical reaction, at different temperatures, comprising: (a) placing a sample in a flat-bottomed container;
- a biochemical sample is located on a filter, membrane, microtitre container or microscope slide in said container, especially a filter.
- the method is programmable and automated.
- the sample is subjected to a pretreatment prior to the method for the sequential reaction.
- a spacer is placed on the filter and a cover plate is placed on the spacer.
- the reaction is a polymerase chain reaction.
- the reaction is for detection of specific DNA sequences.
- the sample is subsequently subjected to a photochemical detection process, especially fluorescence, to detect product of the reaction, and in particular to electronic recording thereof e.g. using a video camera.
- a photochemical detection process especially fluorescence
- a further aspect of the present invention provides rotary thermocycling apparatus especially for biochemical reactions, comprising:
- Fig. 1 is a schematic representation of a rotary thermocycling apparatus of the invention, in plan view;
- Fig. 2 is a schematic representation of the rotary thermocycling apparatus of Fig. 1 , as seen through A-A;
- Fig. 3 is a schematic representation of a front view of the rotary thermocycling apparatus of Fig. 1 ;
- Fig. 4 is a schematic representation of a cross-section of a spray unit
- Fig. 5 is a schematic representation of a cross-section of a sample on a filter within a container.
- the present invention is described herein with reference to a rotary thermocycling apparatus having four stations, each at a pre-determined temperature. This is the preferred number of stations, but is understood that the rotary thermocycling apparatus could have more or fewer than four stations at pre-determined temperatures, depending on the particular use intended for the apparatus. It is understood that, if there were more than four stations, more than one station could have a spray unit.
- the container used in the apparatus will be generally referred to as a dish.
- other examples of containers are disclosed herein.
- Fig. 1 shows a rotary thermocycling apparatus, generally indicated by 1.
- Rotary thermocycling apparatus 1 has floor 2 on which is located rotating table 3.
- Rotating table 3 has four stations viz. first station 4, second station 5, third station 6 and fourth station 7.
- Rotary table 3 rotates about shaft 14, so that a sample is moved in sequence from one station to the next. It is understood that the sample would be suitably located in a dish or other carrier receptacle, which would contact with the heated plate at each station.
- Each location of the stations has a heated plate with each heated plate having means to independently control the temperature thereof at a pre- determined temperature.
- the four stations are located symmetrically around rotating table 3 i.e. at 90° intervals.
- the heated plates are located at fixed locations in floor 2.
- First station 4 has heated plate 10
- second station 5 has heated plate 11
- third station 6 has heated plate 18
- fourth station 7 has heated plate 19.
- the heated plates do not rotate with rotary table 3, but rather rotary table 3 rotates so that each station is located over a heated plate when rotary table 3 is in each position of the sequence.
- Rotary table 3 does not rotate continuously, but moves in steps with a dwell time at each step.
- First station 4 is an open station i.e.
- Lid lifter 9 is located adjacent to second station 5.
- Lid lifter 9 has lid lifter shaft 17 which pivots about lid lifter pivot 12.
- the end of the lid lifter shaft 17 opposed to lid lifter pivot 12 has lid lifter suction cup 13 located thereon.
- Lid lifter 9 is adapted to rotate about lid lifter pivot 12 so that lid lifter suction cup 13 is located above second station 5.
- lid lifter 9 is adapted to move downwards towards second station 5. The operation of the lid lifter is discussed below.
- Each of third station 6 and fourth station 7 has a heating unit associated therewith and which is lowered onto samples at these stations, as discussed herein.
- the heating units are not shown in Fig. 1 (see Figs. 2 and 3), but are attached to supports 28 and 29, respectively.
- Each of the four stations has a heated plate located at the position of the station, as discussed above, that may be controlled at a predetermined temperature.
- the heated plate is most preferably heated using electrical heating. While the temperature of each of the stations may be varied over a wide range, and controlled at such temperature, a typical arrangement of temperature of the heated plates at the four stations is first station 50°C, second station 50°C, third station 72°C and fourth station 96°C. Such temperatures are typical of temperatures for use with polymerase chain reactions, but the temperatures may be varied.
- the apparatus of the present invention preferably has suitable automated control systems, as discussed below.
- Fig. 2 relates to the apparatus of Fig. 1 , as seen through A-A.
- Fig. 2 shows rotary thermocycling apparatus 1 located within housing 20.
- Housing 20 has housing window 21 along the front side of the apparatus, for viewing of the thermocycling apparatus in use.
- Housing 20 has floor 2 located away from the base of housing 20, primarily for the purpose of convenience and for location of motors and other operating parts of the thermocycling apparatus beneath floor 2.
- Shaft 14 extends upwards through floor 2 at a substantially central location, and is connected to drive motor 22 to effect rotation of shaft 14.
- Rotating table 3 is rotated by means of shaft 14.
- Shaft 14 could be adapted to provide support, with suitable bearings, for each of the heating units of the third and fourth stations, and for spray unit 8.
- Second station 5 and third station 6 are shown as being located in rotating table 3.
- Spray unit 8 is located above second station 5 and first heating unit 31 is located above third station 6.
- Second station 5 has heated plate 11 , which is located in floor 2 and is not part of rotary table 3.
- third station 6 has heated plate 18, also in floor 2 and not part of rotary table 3.
- First heating unit 31 is shown in a partially lowered position, as represented by support 15 being in position 15A.
- First heating unit 31 has heating section 23 located on the underside thereof. It will be noted that heating section 23 is of a shape so that central region 24 of heating section 23 will enter into third station 6 while the upper portion of heating section 23 extends beyond the circumference of third station 6. It is intended that heating section 23 would lower to a position such that central region 24 of heating section 23 would enter into third station 6. The purpose of central region 24 entering into third station 6 will be discussed below.
- Second heating unit 32 is located above fourth station 7 in the same manner as first heating unit 31 is located above third station 6.
- Spray unit 8 is located above second station 5.
- Spray unit 8 has lid lifter 9 associated therewith.
- Lid lifter 9 has lid lifter suction cup 13 connected, through lid lifter shaft 17, to lid lifter pivot 12.
- Lid lifter 9 is intended to rotate about pivot 12 so that suction cup 13 becomes located above second station 5.
- lid lifter 9 is then adapted to cause suction cup 13 to descend into second station 5 for the purpose of lifting a cover, 25 (see 64 in Fig. 5), from a sample dish located within second station 5, as discussed below.
- Fig. 2 shows cover 25 located on suction cup 13, but in a position disposed away from second station 5, to permit a spray from spray unit 8 to be sprayed onto a sample in second station 5.
- Spray unit 8 may be of a variety of designs, but is shown in the form of a spray container 26 having a spray nozzle 27. In this embodiment, it is intended that spray container 26 would be an aerosol container or a pump action sprayer, or other type of spraying containing the required liquid reagent(s) to be sprayed onto the sample. A preferred embodiment of spray unit 8 is shown in Fig. 4.
- Fig. 3 shows a front view of rotary thermocycling apparatus 1. This view shows first station 4 and second station 5, with first heating unit 31 of third station 6 located behind second station 5, and second heating unit 32 of fourth station 7 located behind first station 4. Heating section 23 is associated with first heating station 31 and heating section 30 is associated with second heating station 32. Spray unit 8 is shown as located above second station 5. Lid lifter 9 is located beside second station 5.
- Fig. 4 shows a cross section of one embodiment of a spray unit.
- the spray unit shown in Fig. 4 has a spray canister 40 that is connected to a spray head 41 , part of which is spray nozzle 42.
- Spray canister 40 is located between pistons 43 and 44 and held in place by spray holder 45, which is connected to pistons 43 and 44.
- Pistons 43 and 44 are mounted on spray mount 46.
- Piston rod 47 extends from spray holder 45 and terminates in piston plate 48. It will be noted that spray nozzle 42 abuts piston plate 48.
- Spray 49 extends from spray nozzle 42 to contact sample 50. It will be appreciated that a variety of spray units could be used, examples of which are illustrated in Fig. 1 and 2 and in Fig. 4.
- Fig. 5 shows a cross section of a sample in a dish.
- the dish, 60 contains salt pad 61 , which is optional, as discussed herein.
- Filter 62 lies on salt pad 61 and is held in place and separated from cover 64 by spacer 63.
- Spacer 63 is conveniently in the form of an O-ring.
- cover 64 could be in a variety of forms, including a cover insertable into a dish or onto a dish.
- a sample is placed on a suitable carrier for use in the apparatus.
- the carrier is most preferably a filter, with the sample being placed on the filter by standard filtration techniques. For instance, if the particular material to be tested is a solution e.g.
- the filter could be placed in a standard flat-bottomed filtration funnel and the sample filtered to be retained on the filter. This would result in the cells of the particular species to be detected being scattered randomly on the filter, which would facilitate detection at a later stage.
- the sample could be on a membrane, a microscope slide or in a microtitre dish, or in some other suitable form. It is understood that the sample should be substantially planar and of a size that will fit within the dish that is used in the rotary thermocycling apparatus 1.
- the dish referred to herein is any suitable flat bottomed receptacle that will fit within the stations of the apparatus and retain the sample, including cover plates, salt pads or any other item placed within the dish that is related to the reaction being conducted.
- the heating plates associated with the positions of the rotary thermocycling apparatus are heated to predetermined temperatures.
- the first station could be at temperature of 50°C, the second station at the same temperature, third station at 72°C and fourth station 96°C, it being understood that the temperatures are optimized for particular types of reactions.
- the sample is conveniently placed in the first station. If two samples are to be tested at the same time, the unit would be manually turned and the second sample placed in the station opposed to the first station.
- the unit would be manually rotated and samples placed in each of the stations.
- the rotary thermocycling apparatus would preferably have automatic controls to control temperatures, as well as control other parameters relating to the process, particularly the dwell time at each station, the duration and timing of any spray that is used and the number of sequential steps in the reaction.
- the sample is placed in the rotary table at the first station and then rotated to the second station.
- lid lifter 9 rotates over the second station and lid lifter suction cap 13 is moved downwards to contact the cover plate on the sample.
- the suction cup 13 is then retracted and moved out of position, taking with it the cover, and thereby exposing the sample on the filter.
- Piston rod 47 of the spray unit see Fig.
- rotary table 3 rotates so that the sample becomes positioned at the third station.
- heating unit 31 descends onto the sample and into contact with the cover. The sample at this time is heated from below by the heated plate to a pre-determined temperature, for example 72°C, and simultaneously heated from above by the heating unit to the same temperature.
- rotary table 3 rotates to position the sample at the fourth station, at which it is heated from below by the heating plate at this station to a predetermined temperature, for example 96°C, and from above by heating unit 32 to the same temperature. It is understood that the temperatures would be optimized for the particular reaction.
- the sample is then rotated back to the first station, and is cooled to
- the rotary table 3 rotates the sample from the fourth station to the first station, that the rotary table also effect a turning of the sample e.g. by 25-50°. This may conveniently be obtained by means of a ratchet mechanism on the side of the rotary table 3 (not shown).
- the turning of the sample to change the orientation of the sample in rotary table 3 randomises any inconsistencies in, in particular, the spray unit, as well as heating of the sample so that, after a number of cycles, all parts of the sample on the filter are treated to essentially the same conditions.
- Accelerated cooling of the sample between the fourth station, which is at a temperature of for example 96°C, and the first station at a temperature of for example 50°C may be desirable. Such accelerated cooling could involve use of refrigeration, air jets and/or fans between the fourth and first stations.
- a preferred method of cooling is use of a vortex tube, or a ranque vortex tube, to direct a stream of cooling air onto the sample.
- a vortex tube is an EXAIRTM vortex from EXAIR Corporation of Cincinatti, Ohio, which is constructed of stainless steel.
- the filter needs to be made from an inert material i.e. a material that is stable under the conditions of use, especially temperature, which does not affect the sample on the filter.
- a preferred filter is formed from nylon, with a pore size of 0.2 mm. If the dish that is used has a diameter of 92 mm, then the filter is conveniently of a diameter of 90 mm. The sample of bacteria, or other target, becomes trapped between the fibers of the filter (membrane).
- Extraneous extracellular DNA would normally be removed from cells by incubation of the sample with a nuclease solution applied in a fine spray. The nuclease would then be inactivated and denatured by heat.
- Bacterial cells would normally be lysed by a treatment suitable for the expected species. This could include one or more of the following: temperature shock, enzymic digestion and application of a detergent. Removal of extracellular DNA and lysing of bacterial cells would normally take place prior to placing the sample in the rotary thermocycler apparatus.
- the dish contain a pad of salt, particularly an 89 mm diameter glass-fibre filter disc that contains the solutes required for the PCR process.
- the spacer is conveniently a silicone rubber O-ring, having an external diameter of 92 mm.
- the cover is preferably an 89 mm TeflonTM fluoropolymer cover, in the form of a flat disc.
- covers on the samples, which are removed prior to spraying with reagent and then replaced.
- covers could be used, including discs as described herein and lids that fit over the sample container (dish).
- Preferred covers fit closely to but are spaced from samples e.g. by use of O-rings, but also permit heating units to be lowered into contact therewith for purposes of rapid and easy temperature adjustment and temperature control of the sample. All types of covers are generally referred to herein as cover plates but are to be understood to include discs and other types of covers.
- the spray unit is a small aerosol container or pump spray unit containing the liquid reagent(s) for the reaction.
- a small aerosol container of reagent(s) is convenient, as it enables the container to be readily replaced with another container of the same or different reagent(s).
- other types of spray units may be used with the apparatus of the invention.
- more than one spray unit could be used at the same or different stations. For instance, a programmed sequence of at least two different sprays could be used. It is also understood that in some circumstances, the spray(s) could be used in other than each cycle of the apparatus. More than one liquid reagent may be used, either as a combination of reagents in one spray unit, or as reagents in separate spray units that are sprayed simultaneously, in sequence in the same cycle, in different cycles or in some other manner.
- the apparatus has been particularly described herein with respect to manual insertion and removal of the flat-bottom containers onto and from the first station.
- flat-bottom containers could be automatically inserted onto and removed from the first station, to permit more efficient use of the apparatus and the ability of the apparatus to operate essentially unattended by an operator, including overnight, or for other reasons.
- shaft 14 which could be used for support of heating units, spray units or the like.
- shaft 14 is omitted and other means are provided to support heating, spray and other units. Omission of shaft 14 permits rotating table 3 to be a removable table, to permit cleaning of the table and beneath the table and to permit replacement of the table with another table e.g. with stations of different sizes or shapes e.g. square or oval shapes, or to expedite adaption of the apparatus to a different number of stations.
- double-stranded DNA reaction products on the filter may be sprayed with SYBRTM DX reagent from Molecular Probes, Inc. of Eugene, Oregon, USA., or another stain, specific for the double-stranded DNA.
- SYBRTM DX reagent from Molecular Probes, Inc. of Eugene, Oregon, USA.
- the stained clots of double-stranded DNA fluoresce as dots on a dark background under ultra-violet (UV) light.
- a photo image may be captured by an electronic camera and quantitatively analyzed using computer software to give a cell count for the targeted bacteria in the original sample.
- Single-stranded DNA reaction products are tested for hybridization with a single-stranded DNA sequence probe specific to the expected product.
- probes may be readily detected using radio active labels, or labels that induce photochemical reactions e.g. chemiluminescence, or by other methods. This test would allow for authenticity of the PCR product to be checked simultaneously with quantitative analysis.
- the original sample of bacterial cell suspension or other material received for testing will frequently be diluted prior to filtering the sample.
- the count obtained at the end of a test e.g. using fluorescence, will need to be adjusted to reflect any dilution.
- a sample of for example bacterial cells on a filter could be placed on growth medium agar and incubated. The cells would multiply, and the resultant micro colonies would be more readily detected using PCR in the apparatus described herein.
- a mixed population of cells may be tested. In a mixed population, it is possible to detect one or more specific cell types containing the target DNA, so that the presence or absence of such cell types may be detected, while not detecting other cell types that do not contain the target DNA.
- PCR specificity depends primarily on the choice of primers used to prime the target DNA synthesis and the stringency of the reaction conditions e.g. temperature of DNA annealing, concentration of reagents and other factors. This could enable the detection of a carrier of a particular gene, or solely those members of a taxonomic group that act as a carrier of a DNA sequence diagnostic for that group.
- DNA polymerase enzyme is sprayed on the sample during each cycle, or as otherwise programmed in the sequence of steps in the apparatus. Consequently, it may not be necessary to use a heat-stable enzyme that must be sufficiently stable to denaturation temperatures to be active during the entire PCR process. Even if the enzyme were to be fully or partially destroyed at the denaturation temperatures being used, it would be replaced in the next spray step. Thus, it might be beneficial to use a cheaper less heat-stable enzyme, and possibly more of such an enzyme, rather than a more expensive enzyme that would be stable at the denaturation temperatures used in each cycle.
- Klenow enzyme in place of Taq DNA polymerase in a PCR process, with appropriate adjustment of the optimal temperature of use, and obtain acceptable results.
- the present invention has been particularly described herein with reference to PCR, other reactions could be carried out e.g. involving bacteria, DNA fragments in gel profile blots, viruses or the like, provided the samples could be obtained in a suitable form and appropriate occupational health precautions taken if necessary.
- the heating units of stations five and six have an important effect on the rate at which the sample reaches the required temperature, by reducing the depth of space that has to be heated.
- the volume to be heated extends from the cover to the base of the dish, which is simultaneously being heated from below. In the present invention, that volume is small.
- An important aspect of the present invention is that the rate of cycling may be increased, because each station remains at its pre-selected temperature, and it is not necessary to change the temperature of a metal block frequently during each cycle.
- the apparatus and method of the present invention may be used in a wide range of tests. Examples of such tests include detection of the presence of E. coli, Listeria and Salmonella, and other bacteria, using reagents known for use in detection of such bacteria.
- the apparatus and methods of the invention may also be used in other types of tests that require cycling of temperatures and spray of reagents.
- the apparatus and methods could be usable with some metallic catalyst reactions e.g. platinum catalysed reactions using hydrogen peroxide, other reactions that use thermocycling, formation of layered polymer structures in which thin layers e.g. of a thermosetting polymer, are polymerized in each cycle, and in detection techniques that require thermocycling.
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Abstract
Description
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Priority Applications (6)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
DE69918160T DE69918160T2 (en) | 1998-12-07 | 1999-11-02 | TURNING thermocycler |
AU10228/00A AU1022800A (en) | 1998-12-07 | 1999-11-02 | Rotary thermocycling apparatus |
AT99953474T ATE269163T1 (en) | 1998-12-07 | 1999-11-02 | ROTARY THERMOCYCLER DEVICE |
EP99953474A EP1137490B1 (en) | 1998-12-07 | 1999-11-02 | Rotary thermocycling apparatus |
US09/876,428 US6448066B1 (en) | 1998-12-07 | 2001-06-06 | Rotary thermocycling apparatus |
US10/085,904 US20020110899A1 (en) | 1998-12-07 | 2002-02-27 | Rotary thermocycling apparatus |
Applications Claiming Priority (2)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
CA002255850A CA2255850C (en) | 1998-12-07 | 1998-12-07 | Rotary thermocycling apparatus |
CA2,255,850 | 1998-12-07 |
Related Child Applications (1)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
US09/876,428 Continuation US6448066B1 (en) | 1998-12-07 | 2001-06-06 | Rotary thermocycling apparatus |
Publications (1)
Publication Number | Publication Date |
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WO2000033962A1 true WO2000033962A1 (en) | 2000-06-15 |
Family
ID=4163090
Family Applications (1)
Application Number | Title | Priority Date | Filing Date |
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PCT/CA1999/001035 WO2000033962A1 (en) | 1998-12-07 | 1999-11-02 | Rotary thermocycling apparatus |
Country Status (7)
Country | Link |
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US (2) | US6448066B1 (en) |
EP (1) | EP1137490B1 (en) |
AT (1) | ATE269163T1 (en) |
AU (1) | AU1022800A (en) |
CA (1) | CA2255850C (en) |
DE (1) | DE69918160T2 (en) |
WO (1) | WO2000033962A1 (en) |
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Also Published As
Publication number | Publication date |
---|---|
EP1137490A1 (en) | 2001-10-04 |
AU1022800A (en) | 2000-06-26 |
US20020110899A1 (en) | 2002-08-15 |
EP1137490B1 (en) | 2004-06-16 |
DE69918160D1 (en) | 2004-07-22 |
CA2255850C (en) | 2000-10-17 |
US6448066B1 (en) | 2002-09-10 |
CA2255850A1 (en) | 1999-12-21 |
US20020127709A1 (en) | 2002-09-12 |
DE69918160T2 (en) | 2005-07-07 |
ATE269163T1 (en) | 2004-07-15 |
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