US20070020149A1 - Mechanism for connecting plates of a parallel processing fluid handling system - Google Patents
Mechanism for connecting plates of a parallel processing fluid handling system Download PDFInfo
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- US20070020149A1 US20070020149A1 US11/535,223 US53522306A US2007020149A1 US 20070020149 A1 US20070020149 A1 US 20070020149A1 US 53522306 A US53522306 A US 53522306A US 2007020149 A1 US2007020149 A1 US 2007020149A1
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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
- B01L3/00—Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
- B01L3/50—Containers for the purpose of retaining a material to be analysed, e.g. test tubes
- B01L3/502—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
- B01L3/5025—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures for parallel transport of multiple samples
- B01L3/50255—Multi-well filtration
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N1/00—Sampling; Preparing specimens for investigation
- G01N1/28—Preparing specimens for investigation including physical details of (bio-)chemical methods covered elsewhere, e.g. G01N33/50, C12Q
- G01N1/40—Concentrating samples
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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
- B01L2200/00—Solutions for specific problems relating to chemical or physical laboratory apparatus
- B01L2200/02—Adapting objects or devices to another
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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
- B01L2300/00—Additional constructional details
- B01L2300/08—Geometry, shape and general structure
- B01L2300/0809—Geometry, shape and general structure rectangular shaped
- B01L2300/0829—Multi-well plates; Microtitration plates
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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
- B01L2300/00—Additional constructional details
- B01L2300/18—Means for temperature control
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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
- B01L2400/00—Moving or stopping fluids
- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0403—Moving fluids with specific forces or mechanical means specific forces
- B01L2400/0409—Moving fluids with specific forces or mechanical means specific forces centrifugal forces
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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
- 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
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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
- B01L9/00—Supporting devices; Holding devices
- B01L9/52—Supports specially adapted for flat sample carriers, e.g. for plates, slides, chips
- B01L9/523—Supports specially adapted for flat sample carriers, e.g. for plates, slides, chips for multisample carriers, e.g. used for microtitration plates
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N1/00—Sampling; Preparing specimens for investigation
- G01N1/28—Preparing specimens for investigation including physical details of (bio-)chemical methods covered elsewhere, e.g. G01N33/50, C12Q
- G01N1/36—Embedding or analogous mounting of samples
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- Investigating Or Analysing Biological Materials (AREA)
Abstract
A fluid handling system for parallel processing of a plurality of biological samples, the system comprising at least a first plate and a second plate which are stackable together and each include a plurality of corresponding apertures for receiving the biological samples. A biasing mechanism releasably connects the first and second modules together. The biasing mechanism includes at least one electromagnetic coupling element disposed in one of the first and second modules and at least one corresponding magnetic coupling element disposed in the other of the first and second modules. The electromagnetic coupling element is normally engaged to the magnetic coupling element and is disengageable therefrom when the electromagnetic coupling element is energized, such that the first and second modules are disengaged from one another.
Description
- This is a divisional application of U.S. patent application Ser. No. 10/195,309 filed Jul. 16, 2002, the entire contents of the specification of which is incorporated herein by reference.
- The present invention relates generally to a parallel processing fluid handling system, and more particularly to a mechanism for releasably connecting stackable plates of such a system. The parallel processing fluid handling system may be, for example, used for the preparation of cell fraction samples for electron microscopy.
- Biomedical research is requiring more specialised equipment expressly suited for the new demands of burgeoning new fields such as large scale proteomics, which require more automated, parallel processing of complex protocols to be accomplished in reasonable time limits. Proteomics, for example, generally involves the systematic separation, identification and characterization of the proteins present in a given sample of tissue or biological fluid at a given time.
- Certain processes in proteomics research are currently very time consuming, require individual sample preparation, and do not lend themselves to accurate reproducibility. As more research laboratories are taking on a proteomics approach, there is increasing demand for scaling-up traditionally used bench methodology by implementing robotic systems capable of high-throughput preparation and experimentation processing.
- Electron microscopy is often required in proteomics research, especially as proteomics has evolved from a whole cell based approach to an organellar based approach. Using an electron microscope for identification and verification of sub-cellular and protein targets, requires the careful preparation of cell fraction samples to be studied. Electron microscopy is required to validate the purity of the cell fraction sample preparations by morphometry, and to confirm the localization of proteins within isolated organelles.
- The currently employed approach for the preparation of cell fraction samples for electron microscopy involves a time consuming, manual methodology including using a filtration apparatus to deposit the sample onto a filtration membrane, and subsequently exposing the sample to a complex protocol of chemical treatments. Cell fraction samples prepared in this way for electron microscopy must be individually prepared, and take approximately 4 days per sample to complete. This process is overly time and labour consuming, and renders any high-throughput processing of samples impossible.
FIG. 1 shows an electron micrograph image of such a prepared sample. The scale line represents 240 nanometers. - WO 00/72968 published Dec. 7, 2000, discloses a multiple fluid sample processor and system capable of high through put combinatorial processes, chemical synthesis and diagnostic arrays, and biological assays and processing. A multi-layered fluidic array comprises a plurality of micro-sized reservoirs and interconnecting channels. A pressure or vacuum pumping system is used for fluid delivery and removal. The device can include an upper reservoir layer, a center distribution plate, and a lower well plate, all of which are stacked vertically and can be releasably coupled together. The bottom plate containing the samples process through the other layers, is detachable from the other plates, and conveyed to another location for subsequent processing of the samples. This is preferably done by robotic or other automated means.
- It is an object of the present invention to provide an improved mechanism interconnecting modules of a parallel processing fluid handling system.
- There is therefore provided, in accordance with one aspect of the present invention, a biasing mechanism for releasably connecting stackable plates of a parallel processing, fluid handling apparatus, the mechanism comprising: a first plate and a second plate adapted to be stacked together, each plate comprising a plurality of corresponding apertures; at least one mechanical alignment member for aligning corresponding apertures in the plates when said plates are stacked together; and one of the first plate and the second plate comprising an electromagnetic coupling element, and the other of the first plate and the second plate comprising the electromagnetic coupling element being selectively disengageable from the magnetic coupling member when energized, whereby the first and second plates are disengaged from one another.
- There is also provided, in accordance with another aspect of the present invention, a mechanism for releasably connecting stackable modules of an automated system used for parallel fluidic processing of samples, the modules including at least a first module and a second module adapted to be stacked together and each having a plurality of corresponding apertures therein for receiving said fluid samples, the mechanism comprising: at least one electromagnetic coupling element disposed in one of the first and second modules; a magnetic coupling element corresponding to and aligned with each of the at least one electromagnetic coupling elements and disposed in the other of the first and second modules; an actuator operable to select one of an attractively biased configuration and a repulsively biased configuration, the electromagnetic coupling element and the magnetic coupling element being retained together when said attractively biased configuration is selected and being forced away from each other when said repulsively biased configuration is selected; and wherein when the attractively biased configuration is selected the first and second modules are retained together and laterally adjacent ones of said apertures thereof are sealingly isolated, and when the repulsively biased configuration is selected the first and second modules are disengaged from one another.
- There is further provided, in accordance with another aspect of the present invention, a fluid handling system for parallel processing of a plurality of biological samples, the system comprising: at least a first module and a second module being stackable together and each including a plurality of corresponding apertures therein for receiving said biological samples; and a biasing mechanism releasably connecting the first and second modules together, the biasing mechanism including at least one electromagnetic coupling element disposed in one of the first and second modules and at least one corresponding magnetic coupling element disposed in the other of the first and second modules, the electromagnetic coupling element being normally engaged to the magnetic coupling element and being disengageable therefrom when the electromagnetic coupling element is energized such that the first and second modules are disengaged from one another.
- Further features and advantages of the present invention will become apparent from the following detailed description, taken in combination with the appended drawings, in which:
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FIG. 1 is an electron micrograph of a cell fraction sample created using a prior art cell fraction sample preparation process. -
FIG. 2 a to 2 m are schematic cross-sectional views of steps of a method used to create cell fraction samples according to the present invention. -
FIG. 3 a is a perspective view of a primary configuration assembly of the cell fraction preparation apparatus of the present invention. -
FIG. 3 b is a perspective view of a final configuration assembly of the cell fraction preparation apparatus of the present invention. -
FIG. 4 is a perspective view of a fluid transfer plate of the primary configuration assembly ofFIG. 1 a. -
FIG. 5 is an exploded perspective view of a filter plate assembly of the cell fraction preparation apparatus ofFIGS. 3 a and 3 b. -
FIG. 6 is a perspective view of a pumping plate of the cell fraction preparation apparatus ofFIGS. 1 a and 1 b. -
FIG. 7 is a perspective view of a retainer plate of the final configuration assembly ofFIG. 1 b. -
FIG. 8 is a perspective view of a full robotic assembly for the cell fraction preparation apparatus of the present invention. -
FIG. 9 is a control system block diagram for the automation of the full robotic assembly ofFIG. 8 . - The present apparatus is generally a robotic manipulator and fluid handling system for the fully automated, temperature controlled preparation of a plurality of cell fraction samples for electron microscopic examination. It is capable of preparing a plurality of embedded cell fraction samples at the same time using the full range of preparation protocols. Although the device could be adapted for providing any high-volume, parallel processing, fluid sample preparation and handling, the device is preferably intended for cell fraction sample preparation used in proteomics research for the characterization of isolated organelle purity and location of novel and unexpected proteins by quantitative immunolabeling. The present device will significantly increase cell fraction sample preparation throughput by a factor of at least 1,000 compared to current manual cell fraction sample techniques. The integrated design of the present invention permits the automation of a significant number of complex protocols while minimizing stress on the samples. It also assures standardized high quality sample preparation for analysis that is not currently available by any other approach.
- The increasing scope of proteomics efforts requires laboratories to implement and scale traditional “bench” methods to allow for the high-throughput processing of experimental samples. The present device described below permits a plurality of samples, 96 samples in the preferred embodiment shown and described, to be simultaneously prepared, unattended, in a flexible time limit as short as one working day. This eliminates one of the key bottlenecks in proteomics research and provides, for the first time, a standard of reproducibility in sample preparation and evaluation, hitherto unattained. While the samples can be prepared with the present apparatus in a single day, adjustable parameters allow for processing time to be extended if required.
- The automated system of the present invention comprises a core mechanism consisting of four stackable plates or modules, which may be configured in two main configurations for separate chemical processing of up to 96 parallel samples. The modular design of the core mechanism provides the flexibility necessary to automate complex chemical processing protocols as well as integrating with a 5-axis motion control system. The principle components of this core mechanism are illustrated in
FIG. 3 a throughFIG. 7 , and described in detail below. - The four principle components of the core mechanism are: a
fluid transfer plate 14 providing individual fluid reservoirs for each of the 96 samples, afilter plate assembly 12 holding the filter membrane-bound samples throughout processing, apumping plate 16 for vacuum filtration of the cell fraction samples onto the filter membrane and pressure delivery of the processed samples with pressurized air and, aretainer plate assembly 18 including a removably engaged 96 well plate comprising a polymerized embedding solution therein for collection of the processed samples at the end of the automated protocol. - Although the pumping plate is described herein as being a discrete member, it is equivalently conceivable that the pressure plate is in fact integrally formed with the pressure plate as a single unit. In such a case, a nozzle or nozzles would be provided within the integral plate to provide pressurized air or a vacuum source to perform substantially the same function as the pumping plate described herein. Similarly, where ever feasible, other plates could be combined to form integral units. For example, if the fluid transfer plate could be combined into the filter plate, or an integral filter/pumping plate. However, this may only function properly if the pumping plate is capable of providing sufficient pressure to transfer the samples from the filter membrane to the embedding solution in the wells of the retainer plate.
- Two different configurations of the fluid handling apparatus core mechanism are used throughout the automated sample processing protocol, namely a
primary configuration 10 a and afinal configuration 10 b. Theprimary configuration 10 a consists principally of thefluid transfer plate 14, thefilter plate assembly 12 and thepumping plate 16. For thefinal configuration 10 b, thefluid transfer plate 14 is interchanged for theretainer plate assembly 18. In both configurations, three plates are held firmly together throughout processing by eight permanent magnets (four per face) built into the filter plate, which is always located in the center of the configuration. All other plates contain corresponding electromagnets for de-coupling of the plates from the central filter plate assembly. - Referring now to
FIGS. 3 a and 3 b which show the primary and final configurations respectively of the core mechanism of the fluid handling apparatus in more detail. Theprimary configuration 10 a of the fluid handling apparatus' core mechanism comprises generally the centralfilter plate assembly 12 engaged between the upperfluid transfer plate 14 and thelower pumping plate 16. All plates have substantially the same dimensions, and are preferably aligned using mechanical and/or magnetic alignment members. In one embodiment, at least twodowel pins 43 protrude from either side of thefilter plate assembly 12, and are adapted to mate with correspondingholes 45 located in all other plates which are engageable with the central filter plate assembly. Any other similarly effective mechanical alignment members can equivalently also be used. Eightelectromagnets 46, four located on each major surface of thefluid transfer plate 14, the pumpingplate 16 and theretainer plate assembly 18 are magnetically engageable with thepermanent magnets 44 disposed within the filter plate assembly, and shown in more detail inFIG. 5 . Further, all plates can additionally comprise proximity sensors, preferably magnetic ones, embedded therein, which signal proper alignment to a robotic motion controller. All stackable plates have aconnector 38 protruding from a commonminor edge surface 39 of each of the plates. Theconnection members 38 provide a connector for plugging an electrical connection thereto. This provides the necessary signal and power connections for any sensors and switches in each plate. Thefinal configuration 10 b of the core mechanism of the fluid handling apparatus is similar to the primary configuration, with the exception of the interchange of the fluid transfer plate for theretainer plate assembly 18. - Referring to
FIG. 4 , a plurality ofapertures 28, numbering preferably ninety-six in the embodiment shown and described herein, are transversely located in thefluid transfer plate 14. Theapertures 28 extend through the thickness of the plate. Theapertures 28 provide individual fluid reservoirs for each of the ninety-six samples during chemical processing of the samples. Thefluid transfer plate 14 additionally comprises embedded sensors for independently detecting and monitoring the fluid levels in all individual fluid reservoirs formed by theapertures 28. When the fluid reservoirs can therefore be filled until the fluid level sensors in each reservoir indicate that a predetermined desire level has been reach, at which point no further fluid is added. The fluid transfer plate comprises fourelectromagnets 46, adapted to correspond to the fourpermanent magnets 44 disposed on afirst surface 48 of the filter plate assembly. The faces of theelectromagnets 46 are located on the lower surface, not visible inFIG. 4 , of the fluid transfer plate that is to be mated to the filter plate. - The
filter plate assembly 12 inFIG. 5 comprises a filterplate base member 13, having a centralrectangular recess 21 for receiving therein afilter membrane 20,filter plate screen 22 andfilter plate cap 24. The filterplate base member 13 preferably comprises ninety-sixtransversely extending apertures 30 therein, corresponding to and adapted to be aligned with theapertures 28 of the superimposablefluid transfer plate 14. Both theapertures 30 and theapertures 34 of the filter plate cap are formed such that O-rings 33 can be added around each aperture. Thefilter plate cap 24 preferably has O-rings 33 around eachaperture 34 on both the top and bottom surfaces of the cap. All O-rings 33 can be standard O-rings having circular cross-sections. When two layers of O-rings are to be superimposed, such as for examples those sealing eachaperture 30 of the filterplate base member 13 and those on the underside of the filter plate cap, which are to mate to provide sealing with only thefilter membrane 20 and thefilter plate screen 22 therebetween, one set of O-rings preferably is a so called X O-ring, having a generally X-shaped cross-sectional area and are particularly adapted for mating with standard O-rings. All O-rings 33, just like all components of the entire present cell fraction preparation apparatus, can be autoclaved for sterilization. Correspondingapertures 32 and 34 in thefilter plate screen 22 andfilter plate cap 24, also are aligned with themain apertures 30, normally directed with respect to themajor surface 48 of thefilter plate member 13, when thefilter plate screen 22 andfilter plate cap 24 are disposed within therecess 21 of the filterplate base member 13. Thefilter membrane 20 extends between thebase member 13 and the filter plate screen and filter plate cap, such that when thefilter plate assembly 12 is assembled, the plurality of individual samples can be deposited on the filter membrane, without being intermixed with adjacent chemically processed samples. Teflon seals between each element of the filter plate assembly, and between each stacked plate, are preferably used to ensure that each composite fluid passage is well sealed from adjacent passages. Eight permanent magnets, four on the firstmajor surface 48 and four on the opposingmajor surface 50 of thefilter plate member 13, are used to magnetically engage the other stackable plates to the centralfilter plate assembly 12. - Referring now to
FIG. 6 , the pumpingplate 16 can be alternately used as a pressure or vacuum producing member of the fluid handling core mechanism. Specifically, when the core mechanism is in theprimary configuration 10 a, the pumpingplate 16 is used as a vacuum source to draw the samples onto thefilter membrane 20 retained within thefilter plate assembly 12. When the core mechanism is in thefinal configuration 10 b, wherein the fluid transfer plate is replaced with the retainer plate assembly, the pumpingplate 16 is used as an air pressure source to transfer the processed samples from thefilter membrane 20 to the embedding solution contained within theretainer plate assembly 18. The pumpingplate 16 preferably comprises two sets of nozzles, a plurality ofvacuum nozzles 42 and four sideslot pressure nozzles 35, all of which are disposed within arectangular recess 23 in afirst surface 54 of thepumping plate 16. While a plurality ofvacuum nozzles 42 are used, preferably numbering seventy-seven arranged in a 7×11 matrix such that each nozzle lies between the apertures in the filter plate which preferably number 96 in an 8×12 matrix, fewer or even a single nozzle could also theoretically equivalently be used, in order to provide vacuum and pressurized air to the apertures. Thenozzles 42 are internally in fluid flow communication with one of thehose attachments 40, particularly the lower one shown inFIG. 6 , protruding from thesame edge surface 39 from which theconnector 38 extends. Thehose attachments 40, provide inlet and outlet feed passages for the pumping plate, such that either a pressure or vacuum source can be engaged thereto. A pressurized fluid, preferably air, is provided from theside slot nozzles 35, perpendicularly directed with respect to thevacuum nozzles 42.Vacuum nozzles 42 within the centralpumping plate recess 23, permit fluid flow communication between the vacuum house attachment and therecess 23, and consequently between the vacuum source and the apertures of the filter plate. Fourelectromagnets 46 are disposed within the pumping plate on themajor surface 54, adapted to correspond to the location of thepermanent magnets 44 of the centralfilter plate assembly 12, such that the pumping plate can be releasably engaged to thesecond surface 50 of the filter plate. - All
electromagnets 46 of the plates engageable with the filter plate are oriented such that they are normally magnetically attracted to thepermanent magnets 44. This permits the plates to be retained together once stacked, forming a secure separable engagement which prevents the plates from being unexpectedly separated, offer the necessary compression to sufficiently seal the superimposed apertures, and also prevents any fluid flow communication between horizontally adjacent fluid passages by maintaining a seal between the mating flat major surfaces of contiguous plates. When the individuallycontrollable electromagnets 46 on each plate adapted to be engaged to the centralfilter plate assembly 12 are energized, the energized electromagnets counteract the magnetic attractive force between the permanent magnets and the preferably ferrous electromagnets, causing the plates having the energized electromagnets to be disengageable from the central filter plate. This permits the plates to be normally securely retained together, until such time as one plate, such as the fluid transfer plate, is to be disengaged, in which case all that is required is to energize the electromagnets disposed within the fluid transfer plate, causing said plate to be freely disengageable and even slightly repelled from the central filter plate. The inverse procedure is equally possible for the attachment of a plate to the filter plate. - The
retainer plate assembly 18 shown inFIG. 7 comprises a retainerplate base member 17 having a centralrectangular recess 19 formed therein and sized for receiving a multiple-well plate 26. The multiple-well plate, such as a standard 96-well plate, comprises closedbottom apertures 36 which align with and correspond to theapertures 30 of thefilter plate assembly 12. The 96-well plate 26 can be securely retained in therecess 19, such that theretainer plate assembly 18 can be inverted without the well plate falling out. The retainer plate comprises rubber grommet assemblies disposed about the edge of therecess 19, preferably two along each edge, frictionally engage the edges of the 96-well plate 26 to ensure that it is securely retained within therecess 19. In similar fashion with the other outer plates adapted for engagement with thecentral filter plate 12, the retainerplate base member 17 comprises alignment holes 45 for receiving the locating dowel pins 43 of the filter plate assembly,connector 38 andelectromagnets 46 onsurface 52 for magnetic releasable engagement with the central filter plate. - Having described the principal elements of the core mechanism of the fluid handling apparatus, the methodology involved for the parallel preparation of cell fraction samples using the elements of the core mechanism will now be outlined.
- Beginning with the primary stacked
plate configuration 10 a, biological samples are placed, either manually or by an equivalent automated system, into theindividual apertures 28 of thefluid transfer plate 14 of the coupled configuration, using a standard pipette needle for example. The samples can be added into the apertures individually, or in groups of as few as two samples to as many as the number of apertures in the plate. All subsequent manipulations in the processing protocol can be fully automated using a robot as further described below, however the sample processing protocols can equally be manually performed. The process begins by filtering the cellular fraction samples onto thefilter membrane 20, by providing a vacuum from thenozzles 42 of thepumping plate 16 produced by the source engaged to thehose attachments 40. Needle manifolds 74 of therobot arm assembly 72, preferably comprising multi-channels as described in further detail below however they can have as few as a single needle, dispense and aspirate processing chemicals to and from the 96 individual composite fluid reservoirs formed above the filter membrane as required by a known protocol for the preparation of cellular fractions for electron microscopy. Table 1 and Table 2 below outline a sample process protocol, used for with the present invention for the automated preparation of cell fraction samples. During the sample processing performed by such a protocol, the samples and the entire core mechanism is maintained at approximately 4° C. by a thermoelectrically cooledplatform 70, which incubates the samples in the processing chemicals. The ability to accurately control the temperature of the entire core mechanism and consequently the samples, is an important feature of the present invention. Thethermoelectric platform 70 also permits significant temperature variation, being adjustable such that a temperature range of approximately 4° C.-37° C. is possible. Preferably a temperature range of 2° C. to 10° C. is most often used. Cyclic oscillation between various temperatures is equally possible. The cycle of dispensing chemicals, incubation, and aspiration of chemicals is repeated as many times as required to complete the protocol.TABLE 1 Protocols for automated preparation of cellular fractions for electron microscopy. Unless indicated, all manipulations are completed at 4° C. Repeated steps Nn and respective time durations Tn are specified by the operator. Typical total run times range from 8 to 24 hours for completion. Fixation (manual steps): 1. Fixation solution contains: 5% glutaraldehyde, 1 mM cacodylate buffer, pH 7.4 and, 0.1% CaCl2. 2. Add an equal volume of fixative to 2 ml of 100 μg/ml membrane protein and leave overnight. 3. Load 400 to 500 μl of fixed cell fraction samples to each well of the fluid transfer plate. Fixation (automated steps): 1. Filter on Millipore ™ filter type HA 0.45 μm or 0.8 μm. 2. Wash the filter N1 times for time T1 and incubate with 100 mM cacodylate buffer, pH 7.4. Post fixation: (follow one procedure) Procedure I: 1.1 Fix the samples in 2% reduced OsO4 in 100 mM cacodylate buffer, pH 7.4 N2 times and incubate for time T2. 1.2 Wash N3 times and incubate each for time T3 with 0.25 M sucrose cacodylate buffer. 1.3 Rinse N4 times and incubate each for time T4 with 0.1M maleate buffer, pH 5.7. 1.4 Incubate N5 times each for time T5 in 6% uranyl acetate 100 mM maleate buffer, pH 5.7. 1.5 Wash N6 each for time T6 with maleate buffer 1.6 Wash N7 times each for time T7 with cacodylate buffer. Procedure II: 2.1 Incubate N8 each for time T8 in 1% tannic acid in cacodylate. 2.2 Wash N9 times and incubate each for time T9 with 1% sodium sulfate in 100 mM cacodylate. 2.3 Incubate N10 times and incubate each for time T10 in 5% uranyl acetate, 100 mM maleate buffer, pH 5.7. 2.4 Wash N11 times and incubate each for time T11 with maleate buffer. 2.5 Wash N12 times and incubate each for time T12 with cacodylate buffer. Dehydration: 1. Wash with 50% ethanol N13 times and incubate each for time T13. 2. Wash with 70% ethanol N14 times and incubate each for time T14. 3. Wash with 90% ethanol N15 times and incubate each for time T15. 4. Wash with 95% ethanol N16 times and incubate each for time T16. 5. Wash with 100% ethanol N17 times and incubate each for time T17. 6. Wash with Propylene oxide for N18 times and incubate each for time T18. 7. Wash with 1:3 Epon:propylene oxide N19 times and incubate each for time T19. 8. Wash with 1:1 Epon:propylene oxide N20 times and incubate each for time T20. 9. Transfer to preembed block. 10. Incubate with 100% Epon for time T21. 11. Polymerize. -
TABLE 2 Protocol for automated pre-immunolabeling cellular fractions for electron microscopy. Unless indicated, all manipulations are completed at 4° C. Repeated steps Nn and respective time durations Tn are specified by the operator. Typical total run times range from 8 to 24 hours for completion. Light fixation (manual steps): 1. Fixation solution contains: 0.05% glutaraldehyde, 0.1 M cacodylate buffer, pH 7.4. 2. Add the fixative to the pellet (after incubation of cellular fractions with antibody and centrifugation) of 300 μg membrane protein. Mix gently and leave for 30 minutes. 3. Load 400 to 500 μl of fixed cell fraction samples to each well of the fluid transfer plate. Light fixation (automated steps): 1. Filter on Millipore ™ filter type HA 0.45 μm with saline solution (10 mM TRIS, 0.9% NaCl, pH 7.4). 2. Wash the filter N1 times for time T1 with saline solution. Pre-incubation: 1. Wash the filter N2 times for time T2 with 3% BSA/saline solution at 25° C. Gold-complex incubation: 1. Add the gold-complex (0.5 nm) to the samples for time T3 at 25° C. 2. Wash N4 times for time T4 with saline solution. Fixation: 1. Fix the samples N5 times for time T5 in 2.5% glutaraldehyde, 0.1 M cacodylate buffer, pH 7.4. 2. Wash N6 times for time T6 with 0.1 M cacodylate buffer, pH 7.4. 3. Post-fix the samples N7 times for time T7 in 1% reduced OsO4 and 1.5% potassium ferrocyanide. 4. Wash N8 times for time T8 with 0.05 M maleate buffer, pH 6.0. 5. Incubate N9 times for time T9 in 2% uranyl acetate and 0.0125 M maleate buffer, pH 4.2. 6. Wash N10 times for time T10 with 0.05 M maleate buffer, pH 6.0. Dehydration: 1. Wash N11 times for time T11 with 75% ethanol. 2. Wash N12 times for time T12 with 95% ethanol. 3. Wash N13 times for time T13 with 100% ethanol. 4. Wash N14 times for time T14 with propylene oxide. 5. Wash N15 times for time T15 with 1:1 Epon:propylene oxide. 6. Transfer to preembed block. 7. Incubate with 100% Epon for T16. 8. Polymerize. - Once the sample processing protocols have been completed using the core mechanism in the
primary configuration 10 a, the topfluid transfer plate 14 is electromagnetically released from engagement with thefilter plate assembly 12, and is then removed and replaced with theretainer plate assembly 18, inverted such that thewells 36 of the ninety-sixwell plate 26 are open to and aligned with theapertures 34 of thefilter plate cap 24. Theretainer plate assembly 18 can then similarly be magnetically engaged to the filter plate assembly, securing it in place. The entire core mechanism assembly in thefinal configuration 10 b, is preferably then rotated 180 degrees as a unit, preferably about a central axis of the filter plate, such that theretainer plate assembly 18 becomes the bottom-most plate, and both the centralfilter plate assembly 12 and thepumping plate 16 are inverted. The final configuration of three plates is used for delivery of the processed samples to the ninety-sixwell plate 26 containing the embedding compound, such as polymerized Epon. The samples are transferred from theinverted filter membrane 20 to thewells 36 containing the polymerized embedding solution, using pressurized air provided by theside slot nozzles 35 of thepumping plate 16. The plates are electromagnetically de-coupled and the pumping plate and the filter plate are removed. An embedding solution can then be added to all the open apertures of the retainer plate, in order to seal the processed sample between layers of embedding solution. Finally, once the top layer has been polymerized, the ninety-sixwell plate 26 containing the individual processed cell fraction samples can be removed from theretainer plate assembly 18, such that the individual processed samples contained in the embedding solution can be removed, sectioned, and prepared as required for viewing under an electron microscope. - As mentioned above, while the previously described protocols and plate manipulations can be manually performed, the present invention provides a preferable, fully automated robot capable of performing the entire process once the initial biological samples are inserted into the reservoirs defined by the apertures of the fluid transfer and filter plates.
- Referring to
FIG. 8 , the fully automatedrobot assembly 60 comprises principally an electromagneticrobot arm assembly 72, a five-axis motioncontrol system assembly 61 thecooling platform assembly 70 adapted to receive the elements of the core mechanism forming the primary andfinal plate configurations fluids panel assembly 78, all mounted on anunderlying base member 62. Preferably a second fluids panel assembly is also used, fixed to the back side of therail 68. In which case the first fluids panel assembly provides largely air, and the second largely the process liquids. Therobot arm assembly 72, which is actuated to permit 90° rotation relative to therotary table member 75 for convenience, providing the fifth degree of freedom of the five-axis motion control system that would otherwise have four-axis motion control. Therobot arm assembly 72 comprises a fluid handling means 90 including at least oneneedle manifold 74, the fluid handing means 90 being for dispensing and aspirating processing fluids into theapertures 28 of the fluid transfer plate for processing of the samples contained on filter membrane. Therobot arm assembly 72 also comprises an electromagneticplate manipulating member 76 havingelectromagnets 77 thereon, which is capable of grasping and releasing the elements of the stacked plate fluid handling apparatus described above, such that it is adapted for interchanging thefluid transfer plate 14 with theretainer plate assembly 18, for rotating the entire stacked plate assembly about a central axis such that the plates of thefinal configuration 10 b are inverted, and for removing the filter plate assembly and the pumping plate from the retainer plate assembly at the end of the cell fraction sample preparation procedure, such that the ninety-sixwell plate 26 can be removed from theretainer plate assembly 18. Adjacent the thermoelectrically cooledplatform assembly 70 for incubating the samples in the processing chemicals during the sample processing protocol, is engaged awash station 80, adapted for cleaning the interior and exterior surfaces of the individual dispensing/aspiration needles of theneedle manifold assemblies 74, which can aspirate water to ensure an even more thorough wash. - The electromagnetic
robot arm assembly 72 is displaceable and is controlled by the four-axismotion control system 61, comprising two horizontal base rails 64 on which slidemobile supports 66 for an upper transverse horizontal table 68, acarriage 67 horizontally displaceable on the upper transverse table 68 and which retains a vertical table 69 for vertical relative motion therewith, and a rotarytable mounting bracket 73 that is vertically displaceable on the vertical table 69 and comprises arotary table member 75, which retains therobot arm assembly 72 and permits the pivotal motion of the robot arm about a horizontally extending center axis at the center of therotary table member 75.Actuating input member 65 of the upper transverse horizontal table 68 andactuating input member 71 of the vertical table 69, are adapted for moving their respective tables in space, such that coupled X-Y-Z axis motion of therobot arm assembly 72 is provided. The further coupled O-axis rotational motion of the robot arm assembly about the rotating table 75, coupled to the Z-axis, creates four-axis motion control for therobot arm assembly 72 of the fully automatedrobot 60. - The
robot arm assembly 72 preferably also has an actuatedhinging mechanism 79 enabling Φ-axis rotation of the electromagneticplate engaging member 76, thereby being displaceable from a normally vertical position, substantially parallel to the rotarytable mounting bracket 73, to a horizontal position substantially perpendicular therefrom. This enables theelectromagnets 77 of therobot arm assembly 72 to be engageable with the magnets on the plates of the core fluid handling mechanism, in order to be capable of manipulating one or several of the plates. Generally, therobot arm assembly 72 is used in the vertical position when dispensing and aspirating processing fluids, and is used in the horizontal position for plate or plate assembly manipulation. This last rotational axis motion completes the five-axis motion of the entire robot control system. - The
fluids panel assembly 78 that is provided on thebase 62 of therobot 60, and the similar fluid panel assembly included on the reverse of the transverse table 68, can include a plurality of fluid containers, pumps, valves adapted to contain, mix, and supply the air and processing chemicals as required by the sample processing protocols used. As mentioned above, thepanel 78 is generally used for the air, and the other fluids panel mounted directly on the moving transverse table, is used for all the processing fluids. Conduits (not shown) ensure fluid flow communication between thefluids panel assembly 78 and theneedle manifold assemblies 74 of therobot arm assembly 72, such that the necessary processing chemicals can be fed to and received from the individual plate aperture engaging needles. -
FIG. 9 outlines, in block diagram form, the preferred automation controlled processes of the fully automatedrobot assembly 60 described above. The parameters for the processes (e.g.: number of iterations and time duration) are initially set by the operator on the host computer and then downloaded to the motion controller. All subsequent events are driven by the motion controller and its associated digital and analog input/output controls. - There are two levels of control to assure maintenance of sample integrity during automated sample filtration. A vacuum transducer is used to indicate adjustment of a vacuum source flow rate through the pumping plate by way of a proportional solenoid valve. This allows for gentle filtration of the samples. Because the vacuum source is used for several processes, the flow is gated through a direct-acting solenoid valve as well. Additionally, as the cell fraction suspensions are filtered down onto the charged filter membrane, sensors embedded into the fluid transfer plate indicate the individual fluid levels (up to 96) to the motion controller. If the fluid levels are not similar, the motion controller dictates motion control steps to dispense additional buffer into those wells filtering more quickly than the others and try to proceed. If there is repeated failure, the system stalls to allow manual inspection of the problem.
- Processing chemicals are dispensed to the samples via two stepper pumps and several banks of solenoid valves that act as gates to the individual reservoirs of the processing chemicals. Several chemicals are dispensed as progressive proportions of two of the chemicals. Therefore, two pumps and two solenoid valves are actuated simultaneously to mix the two chemicals. As the processing chemicals are being dispensed, there are two levels of control to ensure proper operation of the fluids handling and integrity of the samples. In the first, as fluid is pumped toward the dispensing needles, fluid motion sensors (IR sensors) detect the presence and velocity of the fluid. The motion controller can calculate volume as a check on the system as the geometry of the fluid lines is known. In the second level of fluid handling control, as the fluid is dispensed into the wells of the fluid transfer plate, sensors embedded in the fluid transfer plate indicate to the motion controller whether the appropriate level of fluid in the individual wells has been attained. The process is repeated for as many times it takes to iterate through the sample processing loop of chemical dispensing and aspiration and the cycle of needle washing and drying.
- All automated events except for temperature control are preferably nested within the motion control protocol. The temperature of the four plates is maintained with temperature sensors and thermoelectric coolers located in the walls of the cooling platform. The temperature control operates semi-independently from the motion controller and its associated input/output controls. Signals from the motion controller dictate the “on/off” state of temperature control when the whole robot powered on or off. If the operator dictates that the temperature must change during some portion of the sample processing protocol, the motion controller will deliver a signal to the temperature controller to go to a new temperature set point. Otherwise, the temperature control feedback loop is independent of the motion control loop and any other actuation dictated by the motion controller.
- The other control loops indicated within the block diagram indicate that all controlled processes but temperature are nested within the control loop for robotic motion. Furthermore, the events that take place on an iterated schedule for progressive processing of the samples (processing chemical dispensing, waste aspiration, dispensing needle wash, and dispensing needle dry), are enclosed with the dotted line indicated by “Iterated Processing Sequence”. All other elements, such as plate alignment and sample filtration, occur one time within a sample processing run.
- When spent processing chemicals are removed from the individual wells by way of the aspiration needles, there are two levels of control to assure maintenance of sample integrity during this waste aspiration. A vacuum transducer is used to indicate adjustment of a vacuum source flow rate through the aspiration needle lines by way of a proportional solenoid valve. This avoids aspirating the sample itself. As the vacuum source is used for several processes, the flow is gated through a direct-acting solenoid valve as well. Additionally, as the spent chemical is removed, sensors embedded into the fluid transfer plate indicate the individual fluid levels (up to 96) to the motion controller. If the fluid levels become low, the motion controller dictates motion control steps to stop aspiration from the well(s) and proceed to the following steps.
- After dispensing or aspiration of fluids from the wells of the fluid transfer plate, the exterior surfaces of the needles can be cleaned in the wash station. When the needles are to be washed, the motion controller actuates a small gear pump to replenish the gravity overflow section of the wash station with clean water. The duration of the actuation is dictated by the operator before the processing run begins. In order to remove any excess water droplets from the exterior surfaces of the needles following a wash, the robot delivers the needles to the wash stations drying section. Here, the vacuum source line is opened fully to create an abrupt pressure drop and carry the moisture on the needles away to the waste. A compressor builds the appropriate level of vacuum as indicated by a vacuum transducer (located on the vacuum reservoir). The actuation is completed by actuation of a solenoid valve by the motion controller.
- Sample ejection is accomplished by slowly pressurizing the pumping plate (via the pressure line) and then releasing pressurized air through the solenoid valve in the opposing vacuum line of the pumping plate. A pressure transducer feeds forward a signal to a proportional solenoid valve to allowing an appropriate flow rate of air from the pressurized air source. When the plate has reached the pressure level necessary for sample ejection, the motion controller actuates opening of the solenoid valve for sample ejection.
- Correct plate alignment is achieved with magnets and magnetic sensors embedded in the four plates and in the cooling platform. The magnetic sensors must indicate to the motion controller that they are positioned correctly in order to be able to proceed to the following steps of processing run. If they are not, the motion controller dictates motion control steps to reposition the plates and try to proceed. If there is repeated failure, the system stalls to allow manual inspection of the problem.
- The integrated processing sequence, identified by the boxed area, indicates the iterated events necessary to complete the chemical processing steps. Namely, it includes the dispense, aspiration, wash and dry commands which are produced by the motion controller. Other process and control commands produced by the main motion controller are the temperature, filtration, ejection and robot motion control commands. Various feedback loops permit precise predetermined control of all systems. It is to be understood that the preferred control system setup is included herein as an example, and could be either slightly modified or vastly different, while nevertheless being able to achieve similar results with the fully automated robot assembly.
- In an alternative embodiment, a smaller and more simplified robot is used. This alternative smaller robot does not provide temperature control, and therefore all plate components have significantly reduced mass, and consequently the systems for motion and fluids control are much lighter and more compact. In this case, temperature regulation is achieved by placing the entire automated robotic system within a temperature controlled chamber, which is possible as a result of the compact geometry and reduced mass of the alternative full system permits. Furthermore, electronics and fluids handling are also consequently consolidated and further miniaturized.
- The lack of intrinsic temperature regulation in the alternate system, permits the components to be made from non thermally conductive materials. This allows the sample processing plates of the system to be molded into more intricate geometries using a polymeric (or plastic) material. This significantly reduces weight and costs of all components, and enables simplified mass-production of the components. Additionally, certain components can be disposable. For example, the filter plate is packaged with a pre-loaded filter membrane, the entire sub-assembly being disposable after anywhere from a single to several uses. The low cost of the plastic molded plates permits the inexpensive replacement of all parts, permitting for convenient disposability.
- An alternative method and structure for coupling and compression of the plates is accomplished by using a simplified mechanism, such as a mechanical clamp for example.
- Similar results can also be obtained with several alternative designs. For example, in the first step of sample filtration, multiple samples are loaded onto a surface charged plate having porous wells and separation is completed with a swinging bucket type centrifugation rotor.
- In an alternative embodiment, a single multiple well plate is used throughout the procedure, providing that the material of the plate and the other components are chemically compatible with all the processing fluids of the processing protocol. Multiple reservoirs for each of the processing chemicals are used to progressively wash and incubate the samples, where the filtered samples contained in the filter plate are submerged in progressive baths for predetermined time periods. The same container is also used for embedding the processed samples, arriving at similar processing results as the preferred embodiment described in detail above.
Claims (17)
1. A biasing mechanism for releasably connecting stackable plates of a parallel processing, fluid handling apparatus, the mechanism comprising:
a first plate and a second plate adapted to be stacked together, each plate comprising a plurality of corresponding apertures;
at least one mechanical alignment member for aligning corresponding apertures in the plates when said plates are stacked together; and
one of the first plate and the second plate comprising an electromagnetic coupling element, and the other of the first plate and the second plate comprising the electromagnetic coupling element being selectively disengageable from the magnetic coupling member when energized, whereby the first and second plates are disengaged from one another.
2. The mechanism as defined in claim 1 , wherein the mechanical alignment member is integral with one of the first and second plates.
3. The mechanism as defined in claim 2 , wherein the mechanical alignment member comprises at least two pins which protruded from one of the first and second plates, and matingly engage corresponding holes in the other of the first and second plates.
4. The mechanism as defined in claim 1 , wherein the plurality of apertures correspond to those of a multi-well microplate.
5. A mechanism for releasably connecting stackable modules of an automated system used for parallel fluidic processing of samples, the modules including at least a first module and a second module adapted to be stacked together and each having a plurality of corresponding apertures therein for receiving said fluid samples, the mechanism comprising:
at least one electromagnetic coupling element disposed in one of the first and second modules;
a magnetic coupling element corresponding to and aligned with each of the at least one electromagnetic coupling elements and disposed in the other of the first and second modules;
an actuator operable to select one of an attractively biased configuration and a repulsively biased configuration, the electromagnetic coupling element and the magnetic coupling element being retained together when said attractively biased configuration is selected and being forced away from each other when said repulsively biased configuration is selected; and
wherein when the attractively biased configuration is selected the first and second modules are retained together and laterally adjacent ones of said apertures thereof are sealingly isolated, and when the repulsively biased configuration is selected the first and second modules are disengaged from one another.
6. The mechanism as defined in claim 5 , wherein the actuator energizes the electromagnetic coupling element when disposed in said repulsively biased configuration.
7. The mechanism as defined in claim 6 , wherein the electromagnetic coupling member and the magnetic coupling member are normally retained together, and the electromagnetic coupling element is disengaged from the magnetic coupling member when energized.
8. The mechanism as defined in claim 5 , wherein at last one of the first and second modules is releasably connectable to a manipulating member by one of the electromagnetic coupling element and the magnetic coupling element thereof.
9. The mechanism as defined in claim 5 , wherein when the attractively biased configuration is selected, the electromagnetic coupling element and the magnetic coupling element retain the first and second modules together with a compressive force sufficient to permit static fluid sealing between each of the plurality of apertures in said first and second modules.
10. The mechanism as defined in claim 5 , further comprising at least one mechanical alignment member for aligning corresponding apertures of the modules when stacked together.
11. The mechanism as defined in claim 10 , wherein the mechanical alignment member is integral with one of the first and second modules.
12. The mechanism as defined in claim 11 , wherein the mechanical alignment member includes at least two pins which protruded from one of the first and second modules and matingly engage corresponding holes in the other of the first and second modules.
13. A fluid handling system for parallel processing of a plurality of biological samples, the system comprising:
at least a first module and a second module being stackable together and each including a plurality of corresponding apertures therein for receiving said biological samples; and
a biasing mechanism releasably connecting the first and second modules together, the biasing mechanism including at least one electromagnetic coupling element disposed in one of the first and second modules and at least one corresponding magnetic coupling element disposed in the other of the first and second modules, the electromagnetic coupling element being normally engaged to the magnetic coupling element and being disengageable therefrom when the electromagnetic coupling element is energized such that the first and second modules are disengaged from one another.
14. The system as defined in claim 13 , further comprising at least one mechanical alignment member for aligning said corresponding apertures of the modules when stacked together.
15. The system as defined in claim 14 , wherein the mechanical alignment member is integral with one of the first and second modules.
16. The system as defined in claim 15 , wherein the mechanical alignment member comprises at least two pins which protrude from one of the first and second modules, and matingly engage corresponding holes in the other of the first and second modules.
17. The system as defined in claim 13 , wherein when the first and second modules are engaged together by the biasing mechanism, the electromagnetic coupling element and the magnetic coupling element retain the first and second modules together with a compressive force sufficient to permit static fluid sealing between each of the plurality of apertures in said first and second modules.
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2002
- 2002-07-16 US US10/195,309 patent/US7122155B2/en not_active Expired - Fee Related
-
2003
- 2003-07-16 WO PCT/CA2003/001068 patent/WO2004007076A2/en not_active Application Discontinuation
- 2003-07-16 AU AU2003249804A patent/AU2003249804A1/en not_active Abandoned
- 2003-07-16 EP EP03763547A patent/EP1525054A2/en not_active Withdrawn
-
2006
- 2006-09-26 US US11/535,223 patent/US20070020149A1/en not_active Abandoned
Cited By (3)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US10634601B2 (en) * | 2012-09-19 | 2020-04-28 | Inguran, Llc | Nozzle assembly for a flow cytometry system and methods of manufacture |
US20200271564A1 (en) * | 2015-03-06 | 2020-08-27 | Inguran, Llc | Nozzle assembly for a flow cytometry system and methods of manufacture |
US11668640B2 (en) * | 2015-03-06 | 2023-06-06 | Inguran, Llc | Nozzle assembly for a flow cytometry system and methods of manufacture |
Also Published As
Publication number | Publication date |
---|---|
WO2004007076A3 (en) | 2004-05-21 |
EP1525054A2 (en) | 2005-04-27 |
AU2003249804A1 (en) | 2004-02-02 |
US20060171850A1 (en) | 2006-08-03 |
WO2004007076A2 (en) | 2004-01-22 |
US7122155B2 (en) | 2006-10-17 |
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Legal Events
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STCB | Information on status: application discontinuation |
Free format text: ABANDONED -- FAILURE TO RESPOND TO AN OFFICE ACTION |