The present invention relates to equipment and methods for preparing samples for analysis. In particular, equipment and methods are provided for automated staining of biological samples on microscope slides.
Many tissues do not retain enough color after processing to make their components visible under a bright-field microscope. Accordingly, it is common practice to add color and contrast to tissue components by staining the tissue with various reagents. In the past, the steps of staining a tissue sample for histological or cytological analysis were performed manually, a process that is inherently inconsistent. Inconsistent staining makes it difficult for a Histologist or other medical personnel to interpret slides and to make comparisons between different samples. Thus, a number of devices and methods have been described that serve to automate the staining process and reduce staining inconsistency. Labor costs and the burgeoning demand for anatomical pathology services also are driving the push for increased automation of the staining process.
Prior art devices for automated staining, especially for high volume staining with traditional reagents such as hematoxylin and eosin (H&E), are primarily of a “dip and dunk” type, where racks of slides are automatically lowered into and removed from a series of reagent baths. For example, U.S. Pat. No. 4,911,098 to Tabata describes an automated staining apparatus, where microscope slides holding tissue specimens are dipped sequentially into a large number of chemical solution containers. The slides are mounted vertically in a slide holder basket and a clamp that engages and disengages the basket is used to move the slides from solution to solution. The clamp can include a mechanism to tilt the basket, which aids in removing excess solution before the basket is submerged in the next solution. Additional automated staining devices of the “dip and dunk” type are described in U.S. Pat. No. 5,573,727 to Keefe, U.S. Pat. No. 6,080,363 to Takahasi et al., U.S. Pat. No. 6,436,348 to Ljungmann et al. and U.S. Patent Application Publication No. 2001/0019703, naming Thiem et al. as inventors.
A common shortcoming of the automated “dip and dunk” staining devices is the possibility for cross-contamination of samples that are simultaneously or sequentially introduced into the same solution baths. For example, cells that become dislodged from one slide can settle onto other slides introduced into the same bath. Another problem inherent to these designs is that as slide baskets are transferred from one bath to another, solutions used in later steps of the staining process become contaminated with residual amounts of solutions used earlier in the process. Furthermore, degradation (such as through oxidation) of solution components over time can lead to inconsistent staining unless the solutions are regularly replenished or exchanged, which is a time-consuming and wasteful process that typically disrupts work-flow in these “dip and dunk” type of automated stainers.
Another type of automatic staining apparatus delivers fresh reagents directly to individual slides. For example, U.S. Pat. No. 6,387,326 to Edwards et al. describes an apparatus for staining slides where slides are expelled one at a time from a slide storage device and individually treated at various staining stations as they move along a conveyor belt transport apparatus. Additional devices for automatically staining individual slides are described in U.S. Pat. No. 6,180,061 to Bogen et al., PCT Publication WO 03/045560, naming Tseung et al. as inventors, and U.S. Patent Application Publication No. US2004/0052685 naming Richards et al. as inventors. While such devices can successfully minimize cross-contamination of slides and help ensure that samples are consistently treated with fresh reagent, the individual treatment of slides lowers throughput. Therefore, the throughput of these individual slide staining devices can be problematic for use in primary staining applications (such as H&E staining) where the number of samples processed in a histology laboratory can run into the hundreds or even thousands per day.
What is needed, therefore, is an apparatus and method for consistent, high-throughput staining of microscope slides that also minimizes the potential for cross-contamination between slides. Furthermore, an apparatus and method that can be replenished with fresh reagents without interruption of work-flow is desirable.
An automated system is provided for performing slide processing operations on slides bearing biological samples. The system enables high sample throughput and increased staining consistency while also minimizing the potential for cross-contamination of slides.
In one aspect of the disclosed system, a workstation for performing a step of a staining protocol is not a bath containing a reagent in which several slides are simultaneously immersed. Rather, according to this aspect, a workstation of the system dispenses a reagent to a plurality of microscope slides with minimal transfer of reagent (and contaminants therein) between individual slides. Thus, a workstation according to this aspect minimizes or substantially eliminates the type of cross-contamination of slides that occurs in prior art “dip and dunk” type automated slide staining systems, where contaminants such as dislodged cells can be transferred through the reagent bath from one slide to another.
In one embodiment, the disclosed system includes a slide tray holding a plurality of slides in a substantially horizontal position and a workstation that receives the slide tray. In a particular embodiment, a workstation delivers a reagent to slide surfaces without substantial transfer of reagent (and reagent borne contaminants such as dislodged cells) from one slide to another. In another particular embodiment, the slide tray holding the plurality of slides holds two or more rows or banks of slides, for example, two rows of 4-10 slides each.
In a more particular embodiment, slides are held in a rectangular slide tray in two rows such that their long dimensions are disposed outward from the central, long axis of the tray toward the long edges of the tray. A reagent dispenser in a workstation is positioned above one or more pairs of slides in the opposite rows, and delivers a reagent to one or more slides in one or the other of the two rows, for example, to a pair of slides that are opposite from each other in the two rows. If the reagent dispenser is positioned above fewer than the total number of slides that are held in the tray, the reagent dispenser can move to dispense reagent to other slides in each row of slides, and/or the slide tray can be moved to bring additional slides into position for reagent dispensing. Alternatively, two or more stationary or moving reagent dispensers can be included in the workstation, or one or more manifolds of dispense nozzles can be positioned above the two rows of slides, for example, along the central, long axis of the tray. Nozzles of a reagent dispenser can direct reagent downward and/or upward toward surfaces of slides.
In another particular embodiment, a workstation includes two or more sets of nozzles that are formed or inserted into a movable block that can be moved along the central, long axis of the tray to dispense reagents to one or more slides, for example, a pair of slides disposed toward opposite sides of the tray. Since slides are held in the slide tray so that they are not touching each other, and the slides are held parallel to one another along the direction in which a reagent is dispensed from the nozzles, reagent applied to one slide has a minimal or substantially non-existent chance of reaching another slide and thereby cross-contaminating the slides.
In another aspect, the disclosed system can include one or more workstations where biological samples on slides can be subjected to various treatments including drying, baking, de-paraffinizing, pre-stain prepping, staining, coverslipping and sealing, and combinations thereof. A transporter also is included for moving a slide tray carrying a plurality of slides between the plurality of workstations. Additionally, a fluidics module, a pneumatics module and a control module can be included to deliver reagents, deliver vacuum and/or pressurized gas, and coordinate function of system components, respectively.
In a particular working embodiment, the disclosed system includes a plurality of workstations that are arranged in a vertical stack and a transporter that comprises an elevator configured to move a slide tray between the vertically arranged workstations and an X-Y shuttle table configured to move a slide tray horizontally, such as in and out of a workstation, in and out of the system itself, or in and out of a parking garage. Particular examples of workstations that can be included in the system are a baking or drying station, a de-waxing or de-paraffinizing station, one or more staining stations and a coverslipping station. In a more particular embodiment, a workstation is provided that can perform two or more of de-paraffinizing, staining and solvent exchanging. In even more particular embodiments, such a workstation has a movable nozzle assembly configured to deliver reagents to individual slides held in a slide tray. Workstations according to the disclosure can be modular and include common electrical, pneumatic and fluidic interfaces such that workstation can be easily added or removed to any of several positions within a slide processing system.
In another aspect, a fluidics module is disclosed for automated handling of reagents that can deliver reagents in packaged concentration or in diluted concentration to a workstation without the need to disrupt the delivery of such reagents by the workstation while replacing or replenishing reagents to the system. In more particular embodiments, the fluid-handling module includes a dual chamber fluid pump. The dual chamber fluid pump includes a pump chamber and a dispense chamber where the pump chamber is configured to alternate between vacuum and pressure. The two chambers and a set of valves allow the dispense chamber to be maintained at a constant pressure for dispensation of a reagent to slides even while additional reagent is added to the dispense chamber from the pump chamber. Alternatively, a pump chamber supplying a dispense chamber can further function as a dilution chamber, and a concentrate pump chamber can be added to provide concentrated solutions to the dilution chamber.
The disclosed system is capable of high throughput staining of biological samples on slides without the shortcomings of conventional dip and dunk systems, particularly by eliminating conventional dip-and-dunking de-paraffinizing and/or staining baths, which tend to degrade through oxidation and/or contamination by biological cells dislodged during the de-paraffinizing process. Instead, the disclosed system can employ fresh, clean reagents, thus minimizing the possibility of cell carryover from slide to slide. Moreover, the disclosed system provides for the first time a fully integrated high throughput system for staining slides from the baking step through the coverslipping step, a process that is not performed by any other commercially available system to date.
Further aspects, features and advantages of the disclosed embodiments will be apparent from the following detailed description of the invention, which proceeds with reference to the following drawings.
The following description of several embodiments describes non-limiting examples of the disclosed system and methods to illustrate the invention. Furthermore, all titles of sections contained herein, including those appearing above, are not to be construed as limitations on the invention, rather they are provided to structure the illustrative description of the invention that is provided by the specification. Also, in order to facilitate understanding of the various embodiments, the following explanations of terms is provided.
The singular forms “a,” “an,” and “the” include plural referents unless the context clearly indicates otherwise. Thus, for example, reference to “a workstation” refers to one or more workstations, such as 2 or more workstations, 3 or more workstations, or 4 or more workstations.
The term “biological reaction apparatus” refers to any device in which a reagent is mixed with or applied to a biological sample, and more particularly to any automated device that performs one or more operations on a biological sample.
The term “biological sample” refers to any sample including biomolecules (such as proteins, peptides, nucleic acids, lipids, carbohydrates and combinations thereof) that is obtained from (or includes) any organism including viruses. Biological samples include tissue samples (such as tissue sections), cell samples (for example, cytological smears such as Pap or blood smears or samples of cells obtained by microdissection), samples of whole organisms (such as samples of yeast or bacteria), or cell fractions, fragments or organelles (such as obtained by lysing cells and separating their components by centrifugation or otherwise). Other examples of biological samples include blood, serum, urine, semen, fecal matter, cerebrospinal fluid, interstitial fluid, mucous, tears, sweat, pus, biopsied tissue (for example, obtained by a surgical biopsy or a needle biopsy), nipple aspirates, milk, vaginal fluid, saliva, swabs (such as buccal swabs), or any material containing biomolecules derived therefrom.
The term “code” refers to any type of optical symbology, magnetic pattern or electromagnetic or electrostatic signal containing information. A “code reader” is any type of device that can decipher the information contained in a code. Examples of optical symbologies include characters, barcodes and dataglyphs. Particular examples of barcodes include linear barcodes (such as EAN.UPC, EAN-128, ITF-14 and code 39) multi-dimensional barcodes such as 2D stacked symbologies and 2D matrix symbologies, and composite barcodes such as reduced space symbologies. Even more particular examples of 2D optical symbologies include (p, q) code, PDF417, data matrix, maxicode, vericode, codablock, aztec code, code 16K and QR code. Bar code readers for these and any number of other optical symbologies are well known. Where the code comprises characters (such as alphanumeric characters such as English text and Arabic numbers) the code reader can be an optical character reader (OCR). Magnetic stripes are only one example of a device that can store information in the form of a magnetic pattern. An example of an electromagnetic code is an RFID tag. RFID tags typically include a small metallic antenna and a silicon chip, and can be active or passive. RFID code readers are well known, and typically include an antenna and a transceiver that receives information from the RFID tag. The information content of an RFID tag can be fixed or changeable. In another embodiment, the code reader comprises a CCD camera and the CCD camera can be used for simultaneous detection of slides and reading of a barcode or characters.
The term “organic solvent compatible with coverslipping” refers to a non-aqueous solvent (or mixture of such solvents) that can dissolve a glue (such as on a pre-glued coverslip) used to affix a coverslip to a slide. Examples of such solvents include aliphatic and aromatic hydrocarbons including alkanes (such as branched or straight chain C6-C12 alkanes), terpenes (such as limonene) and benzene derivatives (such as toluene and xylene).
A “plurality” refers to two or more, for example, 3 or more, 4 or more, 5 or more, 10 or more, or even 20 or more.
As used herein, the term “reagent” refers to any liquid or liquid composition used in a slide processing operation that involves adding a liquid or liquid composition to a slide. Reagents include solutions, emulsions, suspensions and solvents (either pure or mixtures thereof). Reagents can be aqueous or non-aqueous. Examples of reagents include solutions or suspensions of antibodies, solutions or suspensions of nucleic acid probes, and solutions or suspensions of dye or stain molecules (such as H&E staining solutions and Pap staining solutions). Further examples of reagents include solvents and/or solutions for de-paraffinization of paraffin-embedded biological samples such as limonene, aqueous detergent solutions, and hydrocarbons (for example, alkanes, isoalkanes and aromatic compounds such as xylene). Additional examples of reagents include solvents (and mixtures thereof) that can be used to dehydrate or rehydrate biological samples, such as ethanol, water and mixtures thereof.
The term “slide” refers to any substrate (such as glass, quartz, plastic or silicon) of any dimensions on which a biological sample is placed for analysis, and more particularly to a “microscope slide” such as a standard 3″×1″ glass slide or a standard 75 mm×25 mm glass slide. Examples of biological samples that can be placed on a slide include a cytological smear, a thin tissue section (such as from a biopsy), or alternatively, can be an array of biological samples, for example a tissue array, a DNA array, an RNA array, a protein array, or any combination thereof. Thus, in one embodiment, tissue sections, DNA samples, RNA samples, and/or proteins are placed on a slide at particular locations.
The term “slide processing operation” refers to any treatment or manipulation of a slide, either with or without a biological sample already placed thereon, or any treatment of a biological sample placed on a slide. Examples of slide processing operations include, but are not limited to, cleaning, heating, cooling, drying, baking, labeling, indexing, removing mercury deposits, re-hydrating, dehydrating, fixing, de-paraffinizing, decalcifying, bluing, digesting, preserving, pre-stain prepping, solvent exchanging, mounting, staining and coverslipping, and combinations thereof.
The term “staining” is used herein to refer to any treatment of a biological sample (such as a cellular smear or a tissue section) that detects and/or differentiates the presence, location and/or amount (such as concentration) of a particular molecule (such as a lipid, protein or nucleic acid) or particular structure (such as a normal or malignant cell, cytosol, nucleus, Golgi apparatus, or cytoskeleton) in the biological sample. For example, staining can provide contrast between a particular molecule or a particular cellular structure and surrounding portions of a biological sample, and the intensity of the staining can provide a measure of the amount of a particular molecule in the sample. Staining can be used to aid in the viewing of molecules, cellular structures and organisms not only with bright-field microscopes, but also with other viewing tools such as phase contrast microscopes, electron microscopes and fluorescence microscopes. Some staining methods can be used to visualize an outline of a cell. Other staining methods rely on certain cell components (such as molecules or structures) being stained without staining the rest of a cell. Examples of types of staining methods include histochemical methods, immunohistochemical methods and other methods based on reactions between molecules (including non-covalent binding interactions), for example, hybridization reactions between nucleic acid molecules. Particular staining methods include, but are not limited to, primary staining methods such as hematoxylin & eosin (H&E) staining and Pap staining, enzyme-linked immunohistochemical methods and in situ RNA and DNA hybridization methods such as fluorescence in situ hybridization (FISH). Additional particular examples of staining methods can be found, for example, in Horobin and Kiernan, “Conn's biological stains: a handbook of dyes, stains and fluorochromes for use in biology and medicine,” 10th ed., Oxford: BIOS, ISBN 1859960995, 2002, and in Beesley, “Immunocytochemistry and in situ hybridization in the biomedical sciences,” Boston: Birkhauser, ISBN 3764340657, 2002.
The term “substantially horizontal” generally refers to an angle within about +/−2 degrees of horizontal, for example, within about +/−1 degree of horizontal such as within about +/−0.8 degrees of horizontal. Substantially horizontal also refers to ranges of small angles from horizontal, for example, angles between about 0.1 degrees and 1.8 degrees from horizontal, such as angles between about 0.2 degrees and about 1.2 degrees, for example angles between about 0.3 degrees and about 0.8 degrees. A slide that is held substantially horizontal will have an orientation such that the large surfaces of the slide are generally facing up and down. In particular embodiments, a rectangular slide such as a microscope slide that is held substantially horizontal will have an angle with respect to horizontal of between about 0.0 degrees and about 2.0 degrees along its short axis and an angle with respect to horizontal of between about 0.0 degrees and 2.0 degrees along its long axis, again with the large surfaces of the slide generally facing up and down. Typically, if a slide has a barcode affixed to one end, a slide held in a substantially horizontal position will have a downward slope away from the barcode along its long axis.
The term “wicking member” refers to any structure (made from any material, for example, metal, plastic or glass) that can break the surface tension of a liquid held on a surface or in a container and facilitate liquid movement off of the surface or from the container. For example, a wicking member such as a small diameter fiber can come in contact with the edge of a slide, and facilitate movement of a liquid from a surface of the slide. A wicking member such as a wicking plate can also contact the edge of a slide tray surface (such as an edge of a bottom or side wall of a slide tray) to facilitate removal of a liquid accumulated in the slide tray. A wicking member is advantageously used in combination with a tilter that lifts a surface away from horizontal such that the surface slopes toward the wicking member. The combination of a wicking member and a tilter can substantially increase the efficiency with which a liquid can be removed from the surface or container.
The term “workstation” refers to a position or location in a disclosed system where at least one slide processing operation is performed, and more particularly to a modular unit inside of which one or more slide processing operations are performed on a plurality of slides held in a slide tray (for example, a plurality of slides held in a substantially horizontal position in a slide tray). A workstation can receive a slide tray in substantially a single position so that movable components of the workstation can locate individual slides within the slide tray and precisely perform a slide processing operation on one or more slides in the tray (such as deliver a reagent to a particular slide or portion thereof). Examples of slide processing operations that can be performed by a workstation include heating, drying, de-paraffinizing, pre-stain prepping, rinsing, solvent exchanging, staining and coverslipping, and combinations thereof. In some embodiments, a workstation dispenses two or more reagents to a slide without the slides being moved from one workstation to another during a slide-processing operation or operations such as de-paraffinizing, staining and/or solvent exchanging. Thus, in one embodiment, a workstation includes a reagent delivery means such as a nozzle or a manifold of nozzles through which reagents are delivered to slides held in a slide tray, which delivery means can be movable or fixed in position within the workstation. Thus, in contrast to some prior art “workstations” which are merely containers holding a reagent in which slides are immersed, a workstation according to the disclosure can be an active, mechanical device that delivers reagents (such as two or more reagents) to groups of slides held together in a slide tray. Thus, in one aspect a work station is not a reagent bath in which slide are immersed. In other embodiments, a workstation can include a heating element and can further include a heat directing element. A heat directing element can help to spread heat more evenly between slides held in a slide tray. A workstation also can include one or more radiant heaters. A workstation also can include a tray tilter (such as a tilt pan) to lift one end of a slide tray to assist with liquid removal from the tray. Alternatively a workstation can include a mechanism to tilt one or more individual slides in a slide tray away from a horizontal position. Workstations can further include various components that move or control other workstation components, such as stepper motors, screw drives and microprocessors. Other components that can be included in a workstation include hoses, belts, tracks, fluidics connections, metering pumps, metering valves, electrical connections, sensors and the like. In another embodiment, a workstation is a modular unit that can be interchanged between two or more positions within a disclosed system and electrically and fluidically connected to the system via a common electronics backplane and a common fluidics manifold. In yet another embodiment, a workstation can include a light source, such as a UV light source for curing an adhesive for holding a coverslip in place on a slide.
Additionally, sensors located at or near reagent supplies for a workstation (or at or near pumps that deliver reagents to a workstation) can monitor reagent volumes in the system and alert a user to a low reagent condition. Furthermore, sensors (such as RFID antennae) can also be used to track reagent data such as reagent identity, amounts and expiration dates to help ensure accurate and consistent reagent use in the system. Overflow conditions in workstations and/or in a waste management system can also be monitored with sensors.
The disclosed staining system can perform all the steps of processing, staining and coverslipping of slide mounted biological samples in an efficient high-speed operation (baking through coverslipping). In a particular embodiment, slides bearing biological samples are placed on a slide tray, and the slide tray bearing the sample slides is loaded into the system. Then, the slides in the slide tray are detected and indexed, and conducted through a sequence of slide processing operations, for example, baking, de-waxing, staining, coverslipping and drying.
In one aspect, the disclosed system is an automated slide processing system that includes a slide tray holding a plurality of slides in a substantially horizontal position (such as in two rows where the slides are held at an angle between about 0.2 degrees and about 1.2 degrees from horizontal) and one or more workstations (for example, arranged in a vertical stack) that receive the slide tray and perform one or more slide processing operations on slides in the slide tray. The workstation can perform a slide processing operation on one or more individual slides in a slide tray, for example, at least two or four slides in a slide tray, or it can simultaneously perform a slide processing operation on all of the slides in a slide tray. In particular embodiments, one or more workstations dispense a reagent to slides in the slide tray without a substantial amount of the reagent that contacts a first slide contacting a second slide, thereby minimizing cross-contamination between slides. Such workstations can include one or more directional nozzles that dispense the reagent onto the slides, for example, the one or more directional nozzles can include a pair of directional nozzles that dispense the reagent in opposite directions across a surface of a slide. In more particular embodiments, the one or more directional nozzles can further include a directional nozzle that dispenses the reagent towards a bottom surface of a slide. In other particular embodiments, the one or more workstations can simultaneously dispense a reagent (for example, the same reagent) to at least two slides held in a slide tray within a given workstation, or the one or more workstations can simultaneously dispense a reagent (such as the same reagent) to all of the slides held in the slide tray within a given workstation.
The disclosed system also can include a transporter to move a slide tray into and out of one or more workstations. Another example of a component or workstation that can be part of the disclosed system is a radiant heater, for example, a radiant heater that has a heat profile that provides substantially uniform heating of slides held in a slide tray positioned below the radiant heater. Yet another example of a workstation is a combined de-paraffinizer/stainer. In a particular embodiment, a combined de-paraffinizer/stainer includes a movable nozzle assembly, wherein the nozzle assembly includes one or more nozzles through which a reagent is dispensed to a slide. The nozzles in the nozzle assembly can be dispense nozzles, forward top surface rinse nozzles that can direct a stream of reagent toward a top surface of a slide (such as at an angle of between about 20 degrees and about 30 degrees relative to the top surface), backward top surface rinse nozzles that can direct a stream of reagent toward a top surface of a slide (such as at an angle of between about 20 degrees and about 50 degrees relative to the top surface), jet drain nozzles, and bottom surface rinse nozzles and combinations thereof. One or more splash guards can also be included on the nozzle assembly as can one or more air brooms or blow-off nozzles.
Yet another type of workstations that can be included in the disclosed system is a coverslipper. Other examples include a drying oven and a solvent exchanger. A transporter that can move a slide tray between workstations also can be included. In more particular embodiments, a workstation can include a slide tray tilter (such as a tilt pan) and a wicking member that facilitates removal of liquids from the slide tray. In conjunction, a slide tray can include an opening in a side wall of the slide tray, wherein the opening in the side wall is contacted by the wicking member in the workstation.
In a more particular embodiment, a disclosed system includes one or more workstations selected from the group consisting of a combined de-paraffinizer/stainer, a drying oven, a solvent exchanger, and a coverslipper, a radiant heater, and combinations thereof. The radiant heater can have a heat profile that provides substantially uniform heating of the slides held in the slide tray.
In another aspect an automated slide processing apparatus is provided that includes a plurality of workstations including a combined de-paraffinizer/stainer, a solvent exchanger, and a coverslipper; a slide tray holding a plurality of slides; and a transporter. The slides can be held substantially horizontal in the tray, and the workstations can be arranged in a vertical stack, such as a vertical stack where multiple workstations are arranged so they are essentially above or below other workstations in the stack. In a particular embodiment, the combined de-paraffinizer/stainer and the solvent exchanger dispense a reagent to slides in the slide tray without a substantial amount of the reagent that contacts a first slide contacting a second slide, thereby minimizing cross-contamination between slides. In more particular embodiments, the combined de-paraffinizer/stainer and the solvent exchanger each can include a movable nozzle assembly can be positioned to dispense a reagent (such as the same reagent) to one or more slides in the plurality (either one at a time in series or simultaneously to any number less than the total number of slides in the tray), or the combined de-paraffinizer/stainer and the solvent exchanger each can simultaneously dispense a reagent (such as the same reagent) to one or more, (for example, all) of the slides in the plurality through a stationary nozzle manifold. In this aspect, the apparatus can further include a radiant heater and/or a drying oven, wherein the drying oven can be a convection oven, such as a convection oven including a heating element and a blower to distribute heat generated by the heating element across the slides held in the slide tray. A dehumidifier can also be included in the system to reduce humidity within a cabinet enclosing at least a portion of the system. Furthermore, a sensor such as code reader for identifying individual slides on the slide tray can be included in the system where one or more slides are marked with a code. Examples of codes that can be used to mark slides include one-dimensional barcodes, multidimensional barcodes, glyphs such as dataglyphs, RFID tags and magnetic stripes. One or more sensors (such as optical sensors) to detect the presence of individual slides (with or without a code) in particular positions within a slide tray can be included in the system, and one or more sensors (such as magnet/Hall-effect sensor combinations) can be included to detect the presence of a slide tray at particular positions within the system. Sensors for detecting individual slides in a slide tray can be used to ensure that reagents are not dispensed to positions in a slide tray where no slide has been placed, thereby reducing wasteful reagent consumption by the system. In a working embodiment, an optical reflectance detector is used to detect slides in the slide tray, and if a slide is detected, a barcode reader is used to read a barcode on a slide.
In a working embodiment of the apparatus, the transporter comprises an X-Y-Z transport mechanism, which can be an X-Y shuttle table carried on an elevator. A counterweight can be attached to the shuttle table by a cable. Either the counterweight can be driven by a lead screw and a stepping motor, or the slide tray can be driven by a lead screw and a stepping motor. In a more particular working embodiment, the cable suspends the counterweight substantially at its center of gravity and the cable also suspends the shuttle table substantially at its center of gravity, thereby reducing moments that could cause binding as they are moved. A sensor (such as an optical or magnetic sensor) on the elevator stepping motor (such as a drive encoder) and or one or more sensors on the workstations can be used for sensing a location of the elevator relative to a workstation in the plurality of workstations. Within one or more workstations, an overflow sensor (such as a thermistor) for detecting a fluid overflow condition can be included.
In a particular embodiment, the solvent exchanger can include a top surface nozzle that is directed to a top surface of a slide during at least a portion of a slide processing operation. It can also include a bottom surface nozzle directed towards a bottom surface of a slide during at least a portion of a slide processing operation. An inline mixer can further be included in the solvent exchanger, as well as one or more blow-off nozzles that can be used for removing and/or spreading solvents from the slides or over the slides, respectively. A metering pump can also be included so that a controlled amount of a reagent fluid is applied to a surface of a slide.
A working embodiment of the disclosed system also includes a cabinet and a powered exhaust for exhausting fumes from the cabinet. A radiant heater also is included where the radiant heater provides a substantially uniform heating profile across the slides held in the slide tray. A portal formed in a wall of the cabinet for loading and unloading slide trays also is provided in the working embodiment, and further, a de-humidifier is added to decrease humidity within the cabinet.
Any workstation included in the disclosed system can further include a pan forming a bottom wall thereof. The pan can further have a gravity drain formed therein and/or an overflow sensor attached thereto such as a thermistor for detecting an overflow condition in the pan.
In a particular embodiment of a slide tray according to the disclosure, individual slides are held in the slide tray spaced from one another in two rows, and, for example, held substantially horizontal. As such, a code reader in some embodiments is positioned to read codes on slides in one row of the slide tray as the slide tray and/or code reader are moved in one direction relative to one another, and the code reader is re-positioned to read codes on slides on the other row as the tray and/or bar code reader are moved in an opposite direction relative to one another.
Since it is desirable that individual slide positions can be accurately located by moving parts within a workstation in order that slide processing operations are performed precisely a workstation (such as a combined de-paraffinizer/stainer, a solvent exchanger, or a coverslipper) can receive a slide tray in substantially a single position. Therefore, a workstation can include a mechanism to hold a slide tray substantially in a single position, for example, one or more springs can be used to hold the slide tray substantially in the single position.
A workstation according to the disclosure (such as a solvent exchanger, a combined de-paraffinizer/stainer or a workstation that functions as a solvent exchanger, de-paraffinizer and stainer) can include one or more nozzles that dispense a reagent to a top and/or bottom surface of a slide held in a slide tray. In some embodiments, the one or more nozzles include one or more backward top surface rinse nozzles, one or more bottom surface rinse nozzles, one or more forward top surface rinse nozzles, one or more dispense nozzles, and one or more jet drain nozzles. The one or more backward top surface rinse nozzles and the one or more forward top surface rinse nozzle can be positioned to deliver a reagent to substantially the same area on a slide. The nozzles can be fixed in position within the workstation or can be movable within the workstation such as on a movable nozzle assembly. In particular embodiments, the backward top surface rinse nozzles and the forward top surface rinse nozzles are positioned to deliver the reagent at an angle between about 20 degrees and about 50 degrees relative to a top surface of a slide and between about 20 degrees and about 35 degrees relative to the top surface of the slide, respectively. An air jet or jets that can be used for mixing of reagents dispensed to a slide surface (see for example, U.S. Pat. No. 5,650,327, which is incorporated by reference herein), an air broom and/or a blow-off nozzle can be included in a workstation. For example, a movable nozzle assembly can include one or more backward top surface rinse nozzles, one or more bottom surface rinse nozzles, one or more forward top surface rinse nozzles, one or more dispense nozzles, one or more jet drain nozzles, one or more air jets, one or more air brooms and/or one or more blow-off nozzles.
A coverslipper according to the disclosure can include a movable coverslipping head, and the coverslipping head can further include an air broom. The coverslipping head also can further include one or more movable pins that hold a coverslip in position on a slide while a hook attached to the head that is holding the coverslip is removed. In one embodiment, a coverslipper includes a movable coverslipping head, wherein the coverslipping head comprises a coverslip gripper that includes a flexible backing plate and a sealing member connected to or integral with a bottom of the flexible backing plate; the coverslipper further comprising a vacuum source communicating with the gripper, and a mechanism for moving the coverslipping head between a source of coverslips and a dispense position where a coverslip is applied to a slide. A cassette for holding individual coverslips for pick-up by the gripper can further be included, and in particular embodiments, the cassette is keyed to prevent misloading in the apparatus. The coverslipper can also include an RFID antennae connected to an RFID tag reader (for example, located elsewhere in the system) and an RFID tag can be included on the cassette.
Slide processing operations performed by the disclosed system and consumables tracking within the system can be controlled by a computer, which can be physically a part of the system control module or connected to the system's control module from another location. In particular embodiments, the disclosed system can employ two or more distinct layers of computer/microcomputer electronics hardware (see, for example,
In some embodiments of the disclosed system, for example, systems having a single combined de-paraffinizer/stainer, the system can process up to about 100 slides per hour. In other embodiments, such as in embodiments having two or three combined de-paraffinizer/stainers or two or three workstations configured to perform steps of de-paraffinization, solvent exchange and staining, the system can process 150 or 200 or more slides per hours, respectively. In some embodiments two or more drying ovens and two or more radiant heaters also are included in the system to increase throughput.
A particular working embodiment of the disclosed automated slide processing apparatus includes a slide tray holding a plurality of slides in a substantially horizontal position; a plurality of workstations arranged in a vertical stack where the plurality of workstations includes a barcode reader, a combined de-paraffinizer/stainer; a solvent exchanger; a drying oven and a coverslipper; a transporter, where the transporter includes an X-Y-Z mechanism, wherein the X-Y-Z mechanism includes an X-Y shuttle table and an elevator in an elevator space; a garage adjacent to the elevator space for storing the slide tray; a radiant heater located above an uppermost parking station in the garage; a cabinet enclosing the plurality of workstations, a dehumidifier for lowering humidity within the cabinet; and a portal through which the slide tray is introduced into or taken out of the apparatus. In a more particular working embodiment, the combined de-paraffinizer/stainer and the solvent exchanger dispense a reagent to slides in the slide tray without a substantial amount of the reagent that contacts a first slide contacting a second slide, thereby minimizing cross-contamination between slides.
In another aspect, the disclosure provide a fluidics module that can be included in the disclosed slide processing system where the fluidics module is configured to allow replenishment of reagent solutions in the system without interruption of workflow in the system. In one embodiment, the fluidics module includes one or more dual chamber reagent pumps, one or more dual chamber dilution and dispensing pumps, and/or one or more single chamber concentrate pumps. Disclosed pump configurations used in disclosed methods of operation can enable uninterrupted delivery of reagents to system workstations, even while reagents are being replenished in the system.
In another embodiment, two or more consumables used by the apparatus during operation are provided in separate packages, wherein the separate packages are keyed (such as color keyed, mechanically keyed, optically keyed and/or electronically keyed) to help prevent misloading of the packages into the apparatus. In addition, separate packages used in the system can include a code (such as an RFID tag) and the apparatus can further include code readers (such as an RFID reader and antennae) located adjacent installation locations of the packages. In a more particular embodiment, a reagent container is provided for containing a reagent (such as a biological stain) for use in a biological reaction apparatus such as the disclosed system. The disclosed container includes a casing having a bottom, sidewalls and a cover, and a collapsible bag compatible with a reagent to be contained therein, held within the casing. The collapsible bag includes a bottom, sidewalls and a top wall configured and dimensioned to substantially fill the casing when expanded (such as when filled with reagent to capacity). The collapsible bag also has a tube sealed to the top wall of the bag and extending into an interior of the bag. The top wall of the casing is keyed to mate with a corresponding key in the biological reaction apparatus. In particular embodiments, the collapsible bag is formed of a flexible polymer such as a laminated material, for example, a three layer laminate. In other particular embodiments, the tube is sealed to the top wall of the casing and typically one end of the tube extends to or near the bottom of the bag. A fitting can be attached to a distal end of the tube, which in particular embodiment includes an elastomeric seal. The elastomeric typically includes a thin material (or septum) that is easily punctured by insertion of a piercing tube mounted on the apparatus. The fitting can be fixedly located under or to the casing lid and the casing cover can include a cutout for providing access to the fitting. A removable sealing tape can be placed over the cutout. In more particular embodiments, the key can include a color code and/or an interference fit. A barcode and/or an RFID tag also can be affixed to an outer wall of the container to, for example, provide information about the contents of the container.
Another aspect of the disclosure is a method for automated processing of a plurality of biological samples on slides where the slides are held in substantially horizontal positions in a slide tray. In one embodiment, the biological samples comprise paraffin-embedded biological samples. The method includes moving the slide tray to a first workstation and automatically staining the samples in the first workstation and/or automatically de-paraffinizing the sample slides in the first workstation and/or automatically solvent exchanging the samples in the first workstation. The method can further include moving the slide tray to a position under a radiant heater and melting paraffin in the biological samples prior to moving the slide tray to the first workstation. Additionally, the method can include moving the slide tray to a second workstation and automatically solvent exchanging the samples through a series of two or more different solvents in the second workstation. The method can yet further include moving the slide tray to a coverslipper workstation and coverslipping the slides in the slide tray in the coverslipper workstation. An alternative embodiment of the method includes moving the slide tray to the first workstation, de-paraffinizing the samples in the first workstation, staining the samples in the first workstation and also solvent exchanging the samples through a series of two or more different solvents in the first workstation. In more particular embodiments, staining comprises H&E staining or Pap staining. In an even more particular embodiment, staining includes dispensing a hematoxylin solution and an eosin solution to the samples. In another even more particular embodiment, staining includes dispensing a hematoxylin solution, an Orange-G solution and an Eosin-azure solution to the samples. The method can further include rinsing the samples (one or more times with a solution or solvent such as a solution of a surfactant and/or buffer, an alcohol/water solution, or an alcohol solvent. The method also can further include bluing the samples.
A schematic diagram of one embodiment of the disclosed slide processing system is shown in
In a particular embodiment of the system shown in
A schematic diagram of another embodiment of system 2 is shown in
Additional components of the embodiment of
Control module 48 of
Cabinet 60 of
A perspective diagram of a working embodiment of the disclosed system is shown in
Furthermore, this configuration permits rapid removal and replacement of individual workstations to aid reconfiguration (such as adding a second combined de-paraffinizer/stainer to increase system throughput potential) and repair (should a workstation fail or need scheduled maintenance). In other embodiments, one or more combined de-paraffinizer/stainers can be operated as combined de-paraffinizer/stainer/solvent exchangers and the solvent exchanger is not included. In such other embodiments, coverslipper 108 can further include heaters to assist in drying of slide trays by, for example, pre-heating the slide trays before they are transported to convection oven 106.
A dehumidifier 114 also is included in the embodiment of
Adjacent to and in front of the transporter/elevator assembly 118 in
Below both the garage, elevator/transporter assembly and the vertical stack of workstations in
On the right side of the lower portion of the system shown in
In operation, system 2 of
Although a particular slide tray can be processed according to any arbitrary user-defined or pre-defined set of operations, a particular sequence of operations includes first taking a slide tray to barcode reader 100 where slides in the tray are detected by optical sensors on a partition between the transporter space and the code reader and any barcodes on detected slides are read by the code reader. The slide tray is then moved to baking station 126 where biological samples on the slides are heated under radiant heater 124. The baking step can be used, for example, to adhere the samples to the slides and/or to melt an embedding material in the sample. It has been surprisingly discovered that baking the slides under radiant heater 124 greatly aids removal of paraffin from paraffin-embedded tissue samples, as it tends to melt and spread the paraffin in the sample across the surface of the slide. The thin layer of paraffin, having greater surface area now that it has spread across the slide, is more easily removed by a paraffin-dissolving solvent such as limonene, making it possible to remove the paraffin with the solvent, without either heating the solvent before it is applied to the slide or after it has been applied to the slide. Once the slides have been baked, the slide tray is moved to combined de-paraffinizer/stainer 102 where the biological samples on the slides in the slide tray are de-paraffinized if necessary and stained. Since many staining protocols make use of aqueous-based solvents, and coverslipping of a sample is best accomplished once water in the sample has been removed, the slide tray is then moved to solvent exchanger 104 where the sample is treated with a series of solvents to remove water and prepare the slides for coverslipping. In an alternative embodiment, solvent exchange also is performed in workstation 102, which can function to de-paraffinize, stain and solvent exchange samples.
It also has been surprisingly discovered that it is possible to apply a controlled amount of a solvent that is compatible with coverslipping (such as limonene) in solvent exchanger 104 and use that solvent in a coverslipping operation once the slide tray has been moved to coverslipper 108, thereby reducing system complexity in a particular embodiment since the coverslipper 108 can be operated without the need to supply it with fluids. Thus, in this particular embodiment, the slide tray is moved from solvent exchanger 104 (with an amount of a coverslipping compatible solvent on its top surface) to coverslipper 108. Once coverslips are placed onto the slides in coverslipper 108, the slide tray can then be moved to convection oven 106 to cure the coverslip onto the slides (at least partially) and also to dry the tray itself (at least partially). A particular advantage of a disclosed system and a method in which slides are cured in an oven after coverslipping (for example, either a convection oven or a radiant oven) is that even if the coverslipping solvent underneath the coverslip is not completely removed, a skin of glue forms around the coverslip, which holds the coverslip in place during subsequent handling by a health care professional such as a pathologist. Processing slides held in a substantially horizontal position aids curing since the large exposed surface area of the slides facilitates quick and efficient removal of solvents from slide surfaces. Once the slides are cured and the tray dried, the slide tray can be moved back to portal assembly 128 for retrieval by a user. Parking garage 122 can be used to store slide trays at any point during the series of slide processing operations, and as is described below, computer control of the sequence of movements/operations can maximize workflow by helping to ensure that workstations are not idle because no slide tray is available for processing therein.
As described previously, a plurality of slides can be held (such as in substantially horizontal positions) in a slide tray. The slide tray may have any shape, and the slides held in a slide tray can be arranged in any manner. In addition, the slide tray can be configured to hold any number of slides, for example, 5 or more slides, 10 or more slides, 20 or more slides, or even 30 or more slides. Several examples of slide trays of different shapes, holding slides in various arrangements, are shown in top view in
A particular embodiment of a slide tray that can be used in the disclosed system is shown in
A second embodiment of slide tray 200 is shown in top perspective view in
A bottom perspective view of the slide tray of
A close-up of slide support pillar 252 is shown in
A drying oven, which includes a thermally insulated compartment and a heat source, can be used to cure slides after coverslipping (to set the coverslips in place and thus prevent their inadvertent removal during slide handling by a user) and to dry slide trays before they are retrieved from the disclosed system by a user. In one embodiment, as shown in
A second embodiment of the drying oven 300 is shown in
As was discussed with respect to
In a particular optional embodiment, aspirated de-paraffinizing reagent is re-circulated by pump 416 and heated in heaters 418 before it is again dispensed from the dispense nozzles 410 in manifold 408. Filter 420 can be used to remove any cells that might become dislodged from the biological specimens on the slides before the reagent is reapplied to the slides, thereby minimizing the potential for cross-contamination of slides. It should be understood, however, that the use of fresh reagent each time a reagent is applied to a slide is the optimal approach.
In a more particular embodiment, optional radiant heater banks 422 also are included in the workstation, and these heater banks can be used to heat up the slides that rest below them when a slide tray is docked in the workstation. As such, the workstation becomes a combined de-paraffinizer and baking station. As mentioned previously, a baking station can melt and spread paraffin in a biological sample over a greater surface area, thereby facilitating its removal. The radiant heater banks 422 can be used alone, or in combination with recirculation and heating in heaters 418. If desired, accumulated paraffin in the reagent stream can be removed from the re-circulating fluid, for example, by skimming the paraffin from the top or bottom of the fluid, depending upon whether the de-paraffinizing reagent is more or less dense, respectively, than the liquefied paraffin.
Pre-heating the slides, i.e., to soften the paraffin, improves the efficiency of the de-paraffinizing step. Depending on ambient conditions and the amount and type of wax, it may be sufficient to apply the de-paraffinizing fluid to the pre-heated slides, let the fluid work for a few seconds or minutes, and then wash the fluid and wax from the slides using, for example, deionized water dispensed from rinse nozzles 412. If necessary, the de-paraffinizing fluid covered slides can be baked for several minutes or more, for example, about 5 minutes, before being washed. Thus, the de-paraffinizing process is enhanced. Moreover, less de-paraffinizing fluid can be used, and it may not be necessary to filter and recycle de-paraffinizing fluid. Rather, the spent de-paraffinizing fluid may be passed directly to drain, or filtered, and then passed to drain.
Various de-paraffinizing agents can be used in the workstation, and can comprise, for example, aqueous-based fluids such as disclosed in U.S. Pat. Nos. 6,544,798 and 6,855,559 (both of which are incorporated by reference herein), including deionized water, citrate buffer (pH 6.0-8.0), tris-HCl buffer (pH 6-10), phosphate buffer (pH 6.0-8.0), FSC buffer, APK wash™, acidic buffers or solutions (pH 1-6.9), and basic buffers or solutions (pH 7.1-14). If desired, the aqueous-based fluid may also contain one or more ionic or non-ionic surfactants such as Triton X-100™, Tween™, Brij, Saponin and Sodium Dodecylsulfate. The de-paraffinizing fluid can be heated, however this is optional, especially if radiant heaters 422 are included in the workstation and employed in the de-paraffinization process. For example, if the embedding medium is paraffin, which has a melting point between 50-57 degrees C., the fluid can be heated to a temperature greater than the melting point of paraffin, e.g. between 60-70 degrees C. Typically, the fluid is heated in the fluid supply. The use of heated aqueous de-paraffinization fluids is described in more detail in U.S. Pat. No. 6,544,798, which is incorporated by reference herein.
Alternatively, any non-aqueous de-paraffinizing fluid such as limonene, xylene or an alkane-based fluid (such as an n-alkane or isoalkane, or a mixture thereof; see, for example, U.S. Provisional Patent Application No. 60/640,477, filed Dec. 30, 2004, which is incorporated by reference herein), or a combination thereof, can be used. While conventional de-paraffinizing fluid such as xylene may be used, one particular de-paraffinizing fluid that has been used in a working embodiment of the disclosed system is D-Limonene, which is a hydrocarbon of the monoterpene group having a molecular formula C10H16. D-Limonene, which has been used in the food and cosmetic industry for many years is non-toxic, and has become a preferred replacement for xylene in pathology laboratories. D-Limonene is commercially available from a variety of sources under various names including Safsolvent (Ajax Chemicals, Auburn, NSW, Australia), Hemo-De (PMP Medical Industries, Los Angeles, Calif.), Histo-clear (National Diagnostics, Manville, N.J.), BDH xylene substitute (BDH Chemicals Ltd., Toronto, Ontario, Canada), and AmeriClear (Baxter Health Care Diagnostics Inc., McGraw Park, Ill.). D-Limonene performs well as a paraffin solvent and cleaning agent, and also may present a reduced fire risk compared to xylene.
As discussed previously, a radiant heater can be used to bake biological specimens onto slides and/or to soften and spread paraffin in paraffin-embedded tissue specimens as an aid to paraffin removal. Although a baking station can be located anywhere in the disclosed system (for example, as a discrete workstation in a vertical stack of workstations) in the particular embodiments of
In a more particular embodiment, the radiant heater is configured to provide substantially uniform heating of slides held in a slide tray. A general method by which the heating profile of a radiant heater can be configured is discussed below using the particular example of a rectangular slide tray holding a plurality of slides in a substantially horizontal position.
In general, in order to radiantly heat a tray full of slides substantially uniformly with a radiant heater of finite size, the temperature of the radiant heater needs to be hotter around the edges than in the center since heat loss from the edges of the heater occurs at a higher rate than in the center of the radiant heater, and because the slides in the center get heat from both sides while the slides near the edges get heat only from one side.
Advantageously the heater is sized to overlap the outer edges of the slides as far as possible, in this case by amount “a”. The heater plate is displaced by distance “c” above the slides. A temperature distribution as a function of X along the heater plate that produces uniform radiant heat flux as a function of Y is desired.
The effective area of a narrow strip on the slide, dY, as seen from X is dY cos(θ), therefore, the radiant heat energy falling on a slide at Y on a strip of width dY from a strip at X on the heater of dX width is:
dq=IdXrdθ cos(θ)
where dq=energy falling on strip dY wide emanating from dX, I=intensity of radiation (and I=k T4), where T is the absolute temperature in Kelvins.
From geometry this can be reduced to:
dq=kT4dXdYc2/[(X−Y)2+c2]
For a fixed value of Y on the slide, dq(Y) is calculated as an integral over all X on the heater (from −a to X max).
A distribution of Tx such that dq(Y) is the same for all Y is desired, i.e., the amount of heat impinging on any part of any slide should be substantially the same. A solution can be found if some temperature distribution is assumed, thereby allowing the equation above to be numerically integrated. A temperature distribution that works well for solving the equation is an error function where the temperature is maximum at “−a” and asymptotically approaches a constant value somewhere inside the edge of the first slide. A similar analysis is then performed to find the heat distribution required in the heater to produce the desired temperature distribution. This also is an error function, but surprisingly can be approximated by a linearly decreasing heat load.
A workstation is provided that can be used to apply one or more reagents to slides during one or more slide processing operations. Since the workstation typically includes one or more nozzles, and more typically one or more banks of nozzles, the workstation is actually a highly versatile workstation that can function not only as a workstation for applying staining reagents to slides, but also for applying de-paraffinizing, wash and solvent exchange reagents or any other type of reagent used in a particular slide processing operation. Thus, the workstation can also be used as a de-paraffinization workstation and/or a solvent exchange workstation. In a working embodiment of the disclosed system, a single workstation functions as a combined de-paraffinizer/stainer, and in another working embodiment, a single workstation functions as a combined de-paraffinizer/stainer/solvent exchanger. In performing each of these functions, multiple reagents can be applied in any particular series to slides held in a slide tray without moving the slides to another workstation.
As was discussed with reference to
Reagents/air are supplied to particular nozzles or sets of nozzles in nozzle manifold 506 (see discussion of
Most biological stains that are commonly used are aqueous or aqueous/alcohol based. Thus, biological samples such as paraffin-embedded tissue samples are first de-paraffinized and hydrated before staining since aqueous-based stains cannot penetrate paraffin and stain tissue components. Conversely, the fluids used to dissolve coverslip adhesives and mount coverslips onto microscope slides are generally immiscible with water. Therefore, after a biological sample has been stained, the water that remains in the sample is first replaced with a non-aqueous based fluid compatible with coverslipping before the sample is coverslipped. This function can be accomplished in a solvent exchanger workstation.
A working embodiment of a solvent exchanger is shown in
As shown in
As mentioned above, the solvent exchanger 600 can be used to exchange residual aqueous fluids from a previous staining step with a non-aqueous fluid that is compatible with a subsequent coverslipping process. Thus, in addition to the components already discussed above, the solvent exchanger can include an inline mixing valve (not shown) that can be used to deliver a series of reagent solutions that gradually transition from water through alcohol to a non-aqueous fluid such as D-Limonene. In a working embodiment, deionized water (which can include a surfactant such as Tween 20), alcohol and D-limonene are provided in bulk (or from a laboratory water deionizer in the case of deionized water) and mixed in the inline mixing valve to provide such transitioning solutions. In a particular embodiment, the mixing is performed under computer control.
A typical succession of solutions that can dehydrate a biological sample and leave a solvent that is compatible with coverslipping on a slide is as follows:
1) 100% water;
2) 75% water/25% ethanol;
3) 50% water/50% ethanol;
4) 25% water/75% ethanol;
5) 100% ethanol;
6) 75% ethanol/25% D-limonene;
7) 50% ethanol/50% D-limonene;
8) 25% ethanol/75% D-limonene;
9) 100% D-limonene.
In a particular embodiment, as a last slide processing operation performed in the solvent exchanger, the slides are blown clean using blow-off nozzles 606 and then a controlled amount of D-limonene is dispensed to the slides in a slide tray. The slide tray is then transported to the coverslipper by a transporter without removing the D-limonene from the slides, and the D-limonene dispensed in the solvent exchanger is used as the coverslipping solvent in the coverslipper. This embodiment will be discussed in more detail below.
As shown in
A blow-off nozzle like the one illustrated in
The disclosed system also can include a coverslipper workstation that receives a slide tray holding a plurality of slides in, for example, a substantially horizontal position, and performs a coverslipping operation wherein coverslips are added to slides held in the tray. In a working embodiment of the disclosed system, the coverslipper is substantially as described in U.S. Patent Application Publication No. 2004/0092024A1, which is incorporated by reference herein. However, modifications of the coverslipper described in the above application and its operation were implemented in a working embodiment of the disclosed system to increase coverslipper precision, decrease coverslipper complexity and increase system throughput.
Also show in
In a particular embodiment, the coverslips applied to slides are coated, on their bottom surface, with a dry, activatable adhesive. The adhesive is activated by a solvent compatible with coverslipping that is placed on the slide (for example, either in a solvent exchanger or a coverslipper). Examples of dry, activatable adhesives include Permount™ (Fisher Scientific, Pittsburgh, Pa.) or ShurMount™ (Triangle Biomedical, Durham, N.C.). U.S. Pat. No. 6,759,011, describes a more particular example of a pre-glued coverslip that can be used in the coverslipper, and is incorporated by reference herein. In an alternative embodiment, glue is applied to slides (such as through dispense nozzles 738) prior to placement of a coverslip onto a slide.
Any means for transporting slide trays between workstations can be employed in the disclosed system. The transport means can include any combination of shuttle tables, conveyor belts, elevators and the like equipped with one or more means to push slide trays off of or to pull slide trays onto the transport means. In a working embodiment, a transporter includes an X-Y shuttle table for moving slide trays horizontally and an elevator for moving the shuttle table up and down vertically within the system. In a working embodiment, an X-Y-Z transporter is used to move slide trays between modular workstations arranged in a vertical stack.
Sensors such as 810 (optical) and 811 (Hall-effect) carried on the X-Y shuttle table can be used to sense, for example: (1) a home or first garage position; (2) one or more workstation positions; (3) a bar code reader position; (4) a portal position or (5) presence of a tray on the shuttle table or in a garage or workstation. The signals from the sensors can be sent to a central processor and used to control workflow in the system. The sensors can be an inductive-type sensor for sensing a magnet or magnets placed in the elevator and/or on the side or bottom of the slide trays. Alternatively, optical sensors can be employed. Finally, encoders may be mounted on the lead screw and/or the stepper motors in the transporter and/or workstations to provide feedback on tray position, workstation mechanism positions and/or transporter position. Such information can also be used to detect system malfunctions such as jams.
The disclosed automated slide processing system also can include a code reader, for example, an optical bar code reader configured to detect and index individual slides in a slide tray. In this particular embodiment, the code reader includes a single code reading mechanism that works in conjunction with the X-Y shuttle table to index and/or detect slides held in two rows on a slide tray. In a working embodiment, a bar code reader workstation is located above a vertical stack of workstations, and a X-Y shuttle table is used to push the slide tray under the bar code reader assembly to read barcodes on slides in one row in the slide tray, and then the bar code reader assembly is moved to detect and index the other row of slides as the X-Y shuttle table is used to pull the slide tray out from under the bar code reader assembly. In an alternative embodiment, the code reader also can move, either alone or in conjunction with the slide tray to bring individual slides below the bar code reader so that the barcodes can be detected.
A bottom perspective view of a working embodiment of a bar code reader assembly 900 is shown in
As mentioned above, an optical detector or detectors that sense the presence of slides in a slide tray (for example, an Omron EE-SPY sensor, Schaumberg, Ill.) also can be used in conjunction with the X-Y shuttle table. For example, by moving a slide tray underneath a detector(s) fixed within the system (such as a location on a partition between a workstation like the code reader and the elevator space of a X-Y-Z transporter), the presence of slides in particular positions in a slide tray can be detected. Such information can be used, for example, to allow workstations to discriminate between positions in a given slide tray that are actually occupied by a slide and those that are empty, thereby allowing the system to skip over empty locations and avoid dispensing costly reagents directly into the slide tray.
Alternatively, each of the slides can be tagged with an RFID tag, in which case the bar code labels can be eliminated and the bar code reader can be replaced by an RFID reader or readers. Slides also can be tagged with magnetic stripes, and a magnetic stripe reader employed in place of the bar code reader. Or, a combination of bar codes and a bar code reader, RFID tags and RFID reader, and/or magnetic stripes and a magnetic stripe reader can be employed in the code reader. It also is possible to include codes on slide trays in addition to the slides they carry so that particular slide trays can be identified within the system.
A Run Time Executive (RTE) software application can be used to sequence and schedule the operations performed by several workstations on microscope slides held in trays.
A basis of actions performed on a tray can be based on an user-selected protocol which, among other things, designates the workstation operations to be performed on slides in a particular tray and the priority of the tray as “STAT” (expedited) or normal. Using this protocol, the RTE prepares an ordered sequence of workstations to be visited. Since there is only one elevator/table in the working embodiment, it can be viewed as a single server with multiple jobs to perform. Where the schedule for this problem can be calculated, it should be noted that the time of addition of trays to the system by a user cannot be predicted. Likewise, users can change the priority of a tray at any time. With these factors in mind, the schedule is determined dynamically prior to the time the elevator/table becomes available for work. Elevator/table “work” consists of a moving tray from point A to point B. Thus, after completing a move, the elevator/table is available. In anticipation of that time, the executive examines each tray in the system and creates a list of possible moves. Referring to
1. First, determine if a tray can be moved. In order to move a tray, it must be either done in a workstation, “almost” done in a workstation (meaning it is estimated to be done by the time the elevator could next go to the workstation), parked and ready for next workstation, parked and ready for removal, or ready to be parked because of an abnormal condition.
2. If the tray can be moved, its next destination must be identified from its planned sequence and checked for availability. A workstation is considered available if it is both empty and operationally ready. If there is more than one of the target workstations available, the workstation that has been waiting the longest is chosen. If the tray's target workstation is not available, then it will either be routed to the parking garage or it will wait in its current workstation depending on the protocol. If the tray can be parked, the executive always chooses the empty parking slot closest to the tray's next target station.
Once the list of all possible moves is prepared, the executive selects the one move to perform. This selection is based on a determined tray priority and in the event of a tie, the time of arrival (TOA) of the tray to the system (i.e. entry time at the portal). The factors making up a tray's priority are as follows:
1. The highest priority is assigned to a tray if it is currently in the slide detect/bar code reading station. This highest priority is assigned because the shuttle table is involved with this station operation and until it has completed and moved the tray to its next station, no other move can be assigned to the elevator/table.
2. The second highest priority is assigned to a tray with a user-designated STAT priority.
3. The third highest priority is assigned to a tray whose protocol requires that it begin the next process within a certain time limit and that time limit will expire if not moved.
4. The fourth highest priority is assigned to a tray that is either in the portal waiting for entry into the system or in the garage waiting to be removed from the system. This priority accommodates the instances where a user is standing by waiting for the instrument.
5. The lowest priority is assigned to any tray that does meet the other four criteria.
The software mechanics of this selection consists of a record in a dynamic array structure that is made for each tray that can be moved. This record contains tray identification, the determined priority, and the tray's TOA. The array is sorted by priority and then TOA and the entry at the top of the list is the tray given to the elevator/table to perform.
The main system computer is responsible for scheduling and coordinating the movement of all slide trays. It also sends commands to system microcontrollers so that they in turn can operate the valves, pumps, motors, heaters and the like at the appropriate times to perform their individual functions within particular modules such as individual workstations and the fluidics module discussed below. Each of the microcontrollers on the several workstations and the fluidics module has a unique address so that they can be identified and individually controlled by the main controller. Communication between the main controller and the several remote modules is accomplished using a serial RS 232 to RS 485 converter which communicates with the microcontrollers through a shared serial bus. The main system or host computer also can include conventional keyboard and mouse inputs and/or a touch screen. The main system computer also can include one or more USB ports and/or an ethernet port, and/or an LCD display, all of which are conventional and commercially available. Accordingly, details of these several conventional inputs and display devices have been omitted.
As mentioned above, each workstation or module can have its own dedicated microcontroller which is networked to the main system controller, which sends high level commands to the individual microcontrollers. The commands can then be interpreted by the workstation microcontrollers, which then operate the valves, motors, pumps, etc. in each module according to a predetermined sequence. Distribution of control functions to the microcontrollers located on the workstations allows particular manipulations taking place in the workstations to be more accurately timed.
For example, in a working embodiment, a combined de-paraffinizer/stainer microcontroller serves as the electrical interface to the combined de-paraffinizer/stainer workstation for controlling valves for applying bulk reagents and stains supplied by the fluidics module (discussed below) to the slides in the tray. The solvent exchanger also can have a dedicated microcontroller for controlling nozzle manifold movement and fluid delivery to slides. Proximity sensors in the workstations can sense the presence of a tray and the home position of the nozzles to provide feedback to the microcontroller so that it can keep track of and control nozzle position and timing of reagent delivery. Similarly a drying oven workstation microcontroller can provide the electrical interface to the station, and proximity sensors in the station sense the presence of the tray and the temperature in the drying oven to provide feedback to the microcontroller during the slide processing operation.
In the coverslipper workstation of a working embodiment, a microcontroller provides the electrical interface to the coverslipper station or module. Glass coverslips are applied to slides under the control of the microcontroller. Vacuum is monitored by the coverslipper controller using a vacuum sensor, and a drop in vacuum can be used by the microcontroller to detect a situation where a coverslipper is attempting to pick up a broken coverslip. The coverslipper station also can include a microcontroller for controlling an air broom for leveling fluid on the slides, for controlling a motor for moving the coverslip cassettes in and out of the coverslipper and for controlling motors that position the coverslipper head over the cassettes and slides held in a slide tray. Proximity sensors in the station sense the presence of the tray, the home position of the transport mechanism and the position of coverslip cassettes.
An automated fluidics module controller provides the electrical interface to the automated fluidics module, bulk fluid pumps, the baking station radiant heater, the transporter and consumable fluid sensors, which in a particular embodiment include RFID tag readers and RFID antennae.
A fluidics module can be included in the disclosed system. In one embodiment, the fluidics module can continuously deliver reagents in packaged concentration, in diluted concentrations and/or in bulk to workstations, even as reagent supplies are being replenished, thereby reducing work flow disruptions. In a more particular embodiment, the fluid motivating components of the fluidics module operate on pressure differentials to achieve continuous availability of reagents for delivery from a dispensing means, even during recharge of the dispensing means. In a working embodiment, high pressure is used to drive recharge fluid from a pump chamber into a lower pressure dispense chamber, and the dispense chamber maintains a particular dispense pressure by back-relieving the high pressure used for recharge of the dispense chamber through an air system pressure regulator. Reagent pumps, reagent dilution systems, DI water and alcohol delivery systems all can be operated according to this method.
In a working embodiment, the fluidics module includes one or more dual chamber reagent pumps 1000 as shown in
Upper manifold 1002 of the dual chamber pump of
In operation, each of the two chambers of the pump is dedicated to a specific purpose. Referring to both
Transfer valve 1024 links pump chamber 1006 to dispense chamber 1008 through lower manifold 1004, and it is the dispense chamber that dispenses fluid to the system. The dispense chamber is under constant low pressure (such as 15 psi) which is maintained through dispense pressure inlet fitting 1014 by a low pressure supply having an air pressure regulator (not shown). Fluid transfer between the two chambers is initiated by the fluid level dropping below the high level switch of fluid level switch 1018. As fluid is dispensed to the system, the transfer valve opens and fluid passes from the high pressure pump chamber into the low pressure dispense chamber to keep the high fluid level switch in the dispense chamber activated. Dispense pressure is maintained by air pressure back-relieving through the air pressure regulator of the low pressure supply. This process continues until the pump chamber reaches its low switch and is recharged. Fluid leaves the dispense chamber through outlet check valve 1022 to prevent drain back from the system. The constant pressure maintained in the dispense chamber makes it possible to deliver reagent on demand without any interruptions while it is being filled from the pump chamber (dispense chamber can be simultaneously recharged while dispensing). Delivery of reagents to the system is not typically interrupted unless the reagent supply (or supplies) is exhausted, and a low level switch event in the dispense chamber serves as a warning that the dispense chamber has not been recharged. To guard the fluidics module in the event of a failure in the system, distribution chambers for pressure, liquid and vacuum can be employed, and sensors can be used to signal an overflow event by detecting the overflow. Valves can be used to purge overflow to waste during an overflow condition.
In addition to reagents that can be supplied to the system in packaged concentrations (such as stains like hematoxylin, eosin, EA and OG) other reagents (such as bluing solutions and wash solutions) can be delivered to the system as concentrates and diluted prior to delivery to a workstation. Thus, another component that can be included in the disclosed system is a dilution and delivery system. In a particular embodiment, the dilution and delivery system is configured to continuously deliver reagents at diluted concentration even as the diluted reagent is being prepared from a concentrated solution. A dual chamber dilution and dispensing pump 1100 is shown in
Dual chamber dilution and dispensing pump 1100 is operated by a method that is similar to that discussed above for the dual chamber reagent pump 1000 of
Transfer valve 1126 connects dilution chamber 1106 to diluted reagent dispense chamber 1108 through bottom manifold 1104, and it is the diluted reagent dispense chamber that delivers fluid to the system. The diluted reagent dispense chamber is under constant low pressure (such as 15 psi) which is maintained through dispense pressure inlet fitting 1116 by a low pressure supply having an air pressure regulator (not shown, but which can be the same or different from the low pressure air supply and air pressure regulator discussed with reference to
Concentrated reagent can be delivered to the dilution chamber of the dual chamber dilution and dispensing pump of
As indicated above, the single chamber concentrate pump of
Referring to
Typically, two boxes or containers of each reagent are installed in the instrument. Thus, when one box is emptied, the system may automatically switch over to a new box, and can alert a user so that the empty box may be replaced by a new box without interrupting system workflow. Reagents used in greater quantities, such as fluids used in a solvent exchanger (such as alcohol) or a de-paraffinizer (such as limonene) can be supplied from bulk fluid containers. Deionized water can be supplied to the system from a deionized water source external to the instrument. Wash reagents and solvent exchange reagents can be made by diluting metered concentrates of surfactant, alcohol and/or Limonene with a solvent such as deionized water.
A shipping container is disclosed that can be directly installed in the disclosed system (or other biological reaction apparatus) as a reagent supply. The container can include a key or keys for minimizing the potential that a user will inadvertently install the container in an incorrect position in the system, helping to ensure that the correct fluids are pumped to workstations in the system. Since the container can be factory filled, the possibility of spillage by a user also is reduced. A means to store reagent data such as a barcode, a magnetic stripe or an RFID tag also can be included on the container. For example, where an RFID tag is included on the container, the disclosed system can read the RFID tag to further check that the fluid has been installed correctly, and the instrument can update the RFID tag during operation of the system to track reagent use. Data regarding the volume of a reagent pulled from the container by a reagent pump (see discussion above regarding fluidics module) is one example of data that can be used to track reagent use, and such data can be used to determine the amount of reagent remaining in a container. When used in conjunction with the pumps of the fluidics module described above, the disclosed containers are not continually stressed by vacuum or pressure, and are thus less likely to rupture.
A disclosed shipping/reagent supply container is shown in
Collapsible, membranous bag 1302 with tube 1304 and fitting 1312 is shown in both its un-filled and filled forms in
Respectively,
Elastomeric seal 1314 serves to seal a filled bag to prevent its contents from leaking out and to prevent outside contaminates from getting in and to act as a septum which can be fractured when the container is installed into an apparatus, thereby allowing the contents of the bag to be extracted. The septum forms a seal around the piercing tube (discussed below) so that a vacuum can be drawn on the interior of the bag during extraction of the liquid from the bag. The septum feature will now be described. Radially inward from face 1332 starts a conical surface 1334 inclined at about 45° from the axis that leads to septum surface 1336 forming a small disk which is flat and perpendicular to the axis. Conical surface 1334 is thicker than septum surface 1336 (about 0.050″ versus about 0.10″ in a working embodiment). The reason the material of this small disk is so thin is to provide a weak area where the seal will fracture when stressed by insertion of a piercing tube, leaving the thicker conical surface 1334 to form a seal around the piercing tube. Outer flange 1338 of elastomeric seal 1314, which fits around the mating surface 1328 of fitting 1312, restrains surface 1332 from being able to move radially inward while a piercing tube is stretching conical surface 1334 and septum surface 1336. An advantage of this embodiment is that the seal can be re-used, that is, the piercing tube can be extracted, and the seal will contract to its original position. While this does not revert to a perfect seal, it does not leave an open hole, but rather a slit. Thus, it can be reinstalled on the same or another piercing tube on the same or a different apparatus, forming a good seal and again allowing liquid to be vacuum extracted.
Cover 1306 of a working embodiment of the disclosed container is shown in more detail in
As shown in
An assembled container is shown in
A piercing tube 1360 is shown in
In a particular embodiment, a system and method for using read/write enabled RFID tags to manage reagents in the disclosed automated slide processing system also is provided. In this embodiment, one or more reagent containers and coverslip cartridges include self-contained read-write memory devices affixed thereto for keeping track of data related to the container or cartridge. The memory device may be a “touch memory” device such as a DS 1985 F516 Kbit add-on touch memory EPROM (Dallas Semiconductor Corporation, Dallas, Tex.) such as disclosed in U.S. Patent Application Publication No. 2002/0110494, which is incorporated by reference herein. However, in one embodiment, lot-controlled consumables (reagents and glass coverslips) have an RFID tag embedded in a label attached to their respective containers. While RFID chip tags may be used, i.e. RFID tags containing a microchip, chipless RFID tags are of significantly lower cost. During the manufacturing and packaging process, product and container-specific manufacturing data can be recorded on both the label and in the embedded RFID tag. In the case of the RFID tag, this manufacturing data can include, for example the following:
1) Catalog or part number,
2) Lot number,
3) Container serial number,
4) Catalog package name,
5) Bulk fluid name for reagents,
6) Volume in milliliters for reagents or coverslip count for glass coverslips,
7) Expiration date, and
8) Manufacturing data (such as date/location of manufacture)
The manufacturing data in the RFID tag typically will be encrypted and then encoded to allow automated transmission error detection and correction before being written to the tag. After the write, the sections of the tag that store this manufacturing data are write-protected to prevent alteration and misidentification.
Once the consumable having an RFID tag is loaded on the instrument, the software can access a consumable's RFID tag through an on-board RFID reader and antennae. (It should be noted that while RFID reader is the common term used for the device, it will be understood that an RFID reader provides both read and write access to RFID tags). Typically, the disclosed instrument will have one antenna at each possible location where a consumable can be loaded. See, for example,
These antennae are connected to the RFID reader through a multiplexor controllable by software commands. Each antenna is designed to only provide access to an RFID tag at its specific location. Thus, the software can switch the RFID-reader to a specific consumable location and read from and write to the RFID tag on that specific consumable whenever required. One suitable RFID tag, which is commercially available is the Tag-it™ HF-1 transponder Inlay Rectangle RFID tag available from Texas Instruments, Dallas, Tex. The RFID tag may be affixed to or incorporated into the fluid container or cartridge and contains information pertaining to the contents of the fluid container or cartridge such as the contents, type, lot number, expiration and related information. The RFID tag enables communication between the container or cartridge and the system processor, thus adding an element of intelligence to the overall system. The RFID tag includes a memory device which can be mounted on the container or coverslipper cartridge. The memory device functions to initiate the system for each new fluid container or coverslipper cartridge that is presented to the system, and to keep track of the fluid or coverslip slide covers remaining. In operation, the memory device is initially read in the information regarding, e.g., type, volume, type, lot number, expiration and related information in the case of the fluid containers, or number and type of coverslips, etc. in the case of a coverslipper cartridge holder. An RFID antenna is positioned behind each of the boxes and also the coverslipper cartridge to read each of the tags and send a signal to the host computer.
During normal tray processing, a Run Time Executive application may access the RFID tags for a variety of reasons. For example, the initial access to each RFID tag typically may be used to confirm the presence of the consumable and that it can be used; i.e., that the contents have not expired. From that point forward, the Run Time Executive can treat the RFID tags as ancillary memory. Using the memory space, the Run Time Executive records the initial date the consumable was used and the identification of the instrument on which it was first registered. Thus, consumables may be moved from instrument to instrument. As the contents of the consumable are used, the memory space is updated with the current estimated remaining or consumed volume or count, along with the date of the last update and the instrument's identification. The Run Time Executive both assesses and maintains this on-board inventory of consumables so sufficiency of the consumables can be ascertained to determine if all trays loaded into the system can be processed. The Run Time Executive also keeps the operator or user informed as to the estimated capacity for slides in terms of consumables, and can automatically reorder reagents from a supplier when reagents are close to being depleted.
Thus, a user is free to remove or replace any consumable on the instrument at any time during processing, or when the instrument is powered off. By using the RFID tag's memory space to store information about the current contents, a previously removed consumable can be re-loaded and the Run Time Executive is able to track the consumable's contents from where it left off. Furthermore, when RFID tags are used during reagent manufacture as described below, and reagents are scanned into an instrument(s) for use therein, it is also possible to track reagent use on a laboratory-wide basis, and enable automatic re-ordering of reagents as a laboratory's supply is depleted, even when the reagents installed on a given instrument are full, but represent the last few remaining in a laboratory.
Lot-controlled consumables (such as reagents and coverslips) can have an RFID tag embedded in a label attached to their respective container, and such labels can be prepared and attached during manufacturing. In one embodiment, the process utilizes a standard PC, a computer program (that can, for example, provide encryption during label preparation), a database, and a device referred to as an RFID printer. The RFID printer simultaneously prints a paper label and writes to a RFID tag, and also is capable of reading RFID tags. Typically, each RFID tag also is uniquely identified by a number. A bar code scanner optionally can be connected to the PC and employed for data entry. This scanner can be connected such that its data is input to the computer via the keyboard. The process described below is an exemplary sequence of steps that can be used during reagent manufacture:
Prior to starting the computer application, the user loads the RFID Printer with a sufficient quantity of labels/tags. The labels/tags are in a roll and the RFID Printer advances the roll one label/tag at a time. The user then starts the computer program (also referred to as the application) and logs in. The user's name and password are confirmed in a database table so that only authorized users can proceed. The user identifies the product for which labels and RFID tags are to be prepared, including both the product's catalog number and the specific manufacture lot number. This information is keyed into a form presented on a screen by the application. Alternatively, this information can be in bar code form and scanned with a bar code scanner.
The application reads product data from the database using the entered catalog number as a unique database key. Product data can include the catalog package name, the product's bulk fluid name for reagents or coverslip name for coverslips, the package's volume in milliliters for reagents or coverslip count for coverslips, date of manufacture, product expiry date, the usable period of the product after date of first use (such as in units of days), the label type etc. In addition, the application can determine the last container serial number used by accessing container data stored in the database, and if none is found, the last container serial number is initialized to zero. The user then enters the quantity of labels and tags to prepare—one for each container. Alternatively, this quantity can be in bar code form and scanned with a bar code reader.
The application loop then can perform each of the following sub steps until the desired quantity of labels and tags have been prepared:
1. Compute the next container's serial number by adding the loop counter to the last container serial number as determined from the database.
2. Using the RFID Printer, read the unique identification number of the RFID tag in the current print position.
3. Assemble the data to be written to the RFID tag. Exemplary types of product/container data are catalog number, lot number, container serial number, catalog package name, bulk fluid name for reagents, volume in milliliters for reagents or coverslip count for coverslips, usable period in days, expiry, and manufacture date.
4. Encrypt the data using the RFID tag's unique identification number as the encryption key. This helps prevent production of unauthorized copies of an RFID tag and ensures data integrity between the physical labels and the database.
5. Encode the encrypted data using an error correction encoding scheme (such as a Reed-Solomon error correction encoding scheme). This helps ensure reliable data transmission from the RFID tag to the instrument on which the container is installed.
6. Assemble data to be printed on the label. The specific data are listed below.
7. Combine the label data and the tag data into a single data packet.
8. Send the data packet, along with appropriate commands, to the RFID Printer. This causes the label to be printed, the tag to be written and write-protected, and the label/tag to be advanced one print position. The label type is not printed, but is used to trigger the printing of graphics stored in the RFID Printer's memory that are specific to the product.
9. Write a record to the database which represents the physical container, such record containing product/container data and timestamp.
10. The application then cycles back to Step 3 to allow the user to enter data for other containers.
In a particular embodiment, non-toxic waste solvents such as limonene and ethanol can be emulsified and disposed of through a drain to a municipal water treatment plant. A mechanical emulsification apparatus that can be included in the disclosed system is shown in
As illustrated in
Another method that can be performed to remove reagents from individual slides is to tilt the slide themselves. A particular system and method for lifting slides is shown in
Multiple microcontrollers that serve as the interface between the main PC and the low level system functions can be connected to the main computer (for example, via a shared serial RS485 communications bus). Microcontrollers can be allocated between system components, for example, one microcontroller can be allocated to each of several components (such as to each of several workstations, for example, each of a combined de-paraffinizer/stainer, a solvent exchanger, and a coverslipper) or allocated to multiple components or subcomponents (such as a portal and an elevator of a transporter). Such microcontrollers, also known as an IRIS (Independent Remote Input/Output System) can manage the electrical and electromechanical devices within a given system module, workstation or component. A third layer of microcomputer hardware can be implemented where fast and precise mechanical motion is desired (such as for controlling a movable nozzle assembly). The third layer can include a microstepping motor controller, which includes a dedicated microcontroller and a motor driver that moves a stepping motor in response to serially transmitted commands from the IRIS.
While it is possible to add interface PC boards to a PC to directly connect low level devices such as valves and motors, the separation and isolation of the PC and the low level devices with the IRIS relieves the PC of the burden of low level functions such as fast valve operation and motor microstepping. Separation of the functions helps to increase timing accuracy at the device level since clock functions in the IRIS are not disrupted by other tasks as they can be in a PC. In a working embodiment, the PC delivers sets of instructions for controlling system components in the form of a macro that is used by the IRIS to control lower level functions of system components. The PC can also be connected to a larger laboratory information system (such as the Ventana Lab Manager and/or the Ventana Interface Point, Ventana Medical Systems, Inc, Tucson, Ariz.).
In a working embodiment, an IRIS includes a single printed circuit board employing a microcontroller (such as Microchip Corporation part number PIC18F452, Chandler, Ariz.) with sufficient memory and speed to:
1. Communicate with the main PC over a serial communications link.
2. Operate up to twenty-four valves, DC motors, relays or similar devices.
3. Monitor up to twenty digital devices, such as optical and Hall-effect proximity sensors.
4. Monitor up to eight analog devices such as pressure and temperature sensors.
5. Control up to four stepping motors, each via its own serial communications link.
6. Monitor the output of a motor encoder circuit (a second microcontroller on the IRIS can be dedicated to this function) to confirm the rotation of the stepper motors under its control.
A working embodiment of a microstepping motor controller similarly employs a microcontroller (such as Microchip Corporation part number PIC18F258, Chandler, Ariz.) which accepts motor move commands from the IRIS. The motor controller desirably has sufficient speed and computing power to microstep a motor at step rates of up to 16,000 steps per second, and can accurately control acceleration and deceleration of an inertial load without step loss.
In one aspect, an automated slide processing system is disclosed that includes at least one slide tray holding a plurality of slides in substantially horizontal positions and one or more workstations that receive the slide tray and perform a slide processing operation on a slide in the slide tray while the slides remain in substantially horizontal positions. In particular, a workstation in the system can dispense a reagent to slides in the slide tray without a substantial amount of the reagent that contacts a first slide contacting a second slide, thereby minimizing cross-contamination between slides, and the system can further include a transporter to move the slide tray into and out of the one or more workstations. In particular embodiments, the one or more workstations can include a radiant heater, a combined de-paraffinizer and stainer, an automated coverslipper, a drying oven, a solvent exchanger and/or a combined de-paraffinizer/stainer/solvent exchanger. Where two or more workstations are included in the system, they can be arranged in a directly vertical stack.
In one particular embodiment, a system is disclosed for complete processing of slides from baking through coverslipping. Such a system includes a plurality of workstations including a combined de-paraffinizer/stainer/solvent exchanger, a radiant heater, a drying oven and a coverslipper, at least one slide tray holding a plurality of slides in substantially horizontal positions, and a transporter for moving said slide tray between said plurality of workstations.
In another aspect a method is disclosed for automated processing of a plurality of biological samples on slides wherein the slides are held in substantially horizontal positions in a slide tray. Such a method includes moving the slide tray to a first workstation, staining the samples on the slides in the first workstation, moving the slide tray to a second workstation, and coverslipping the slides in the second workstation. Moving the slide tray can include moving the slide tray with an X-Y-Z transporter, and the slides can remain in substantially horizontal positions in the slide tray throughout processing by a workstation(s).
In a particular embodiment, the disclosed method can further include de-paraffinizing the samples in the first workstation, for example, by delivering a de-paraffinizing fluid such as limonene to the samples. In other particular embodiments, staining can include dispensing a hematoxylin solution and dispensing an eosin solution to the samples, or dispensing a hematoxylin solution, dispensing an Orange-G solution and dispensing an Eosin-azure solution to the samples. In addition, the method can further include dehydrating said samples at any time, but particularly between dispensing the hematoxylin solution and dispensing the Orange-G and Eosin-azure solutions to samples.
In yet another particular embodiment, the method can further include moving the slide tray under a radiant heater prior to moving the slide tray to the first workstation and melting paraffin in the samples held under the radiant heater.
In some particular embodiments, the method can further include solvent exchanging said samples through a series of two or more different solvents or solvent mixtures in the first workstation. Solvent exchanging can include dehydrating the samples, rehydrating the samples, or both, in any order one or more times. In still other particular embodiments, the method further includes moving the slide tray to a third workstation and solvent exchanging the samples through a series of two or more different solvents or solvent mixtures in the third workstation. As before, solvent exchanging can include dehydrating the samples, rehydrating the samples, or both, in any order, one or more times.
In other embodiments, the method further includes moving the slide tray to a third or fourth workstation and drying the samples in the third or fourth workstation. In addition, the method can include heating the slide tray in the second or third workstation prior to moving the slide tray to the third or fourth workstation for drying.
In particular embodiments, the method can further include prioritizing any given slide tray, thereby completing all operations on that slide tray first. And in other particular embodiments, the method can include communicating tray status to a laboratory information system. In other particular embodiments, the biological samples include cytological samples, and in yet others, the biological samples can include tissue sections. Of course a mix of different types of biological samples can be included on a particular slide or between different slides held in a particular slide tray.
In yet another aspect, a reagent container is disclosed for containing a reagent (for example, a reagent such as a biological stain, a rinse, a de-paraffinizing fluid, a solvent or a solvent mixture) for use in an automated biological reaction apparatus such as an automated stainer, or any type of automated system for the treatment or processing of biological samples. The disclosed container includes a casing having a bottom, sidewalls and a cover, a collapsible bag compatible with a reagent to be contained therein, held within the casing, the collapsible bag including a bottom, sidewalls and a top wall configured and dimensioned to substantially fill the casing when expanded, the collapsible bag also having a tube sealed to the top wall of the bag and extending into an interior of the bag, wherein said top wall of the casing is keyed to mate with a corresponding key in said biological reaction apparatus. Typically, the collapsible bag is formed of a flexible polymer or some type of laminated material such as a three-layer laminate. Also typically, the tube is attached in some manner to the top wall of the casing, and the tube extends to or near said bottom of the bag. A sealing fitting can be attached to a distal end of the tube, for example, an elastomeric seal can be attached to the distal end of the tube. Such an elastomeric seal con include a thin material that is easily punctured by manual insertion of a piercing tube. The fitting can be fixedly located under or to the cover, and the cover and or a sidewall can include a cutout for providing access to the fitting. A removable sealing tape can be placed over the cutout, for example, to protect the fitting and its seal during shipping.
In a particular embodiment, the container can be keyed, such as with a color code or an interference fit (for example, a protrusion or shape that permits insertion of the container into one or more particular positions in a biological reaction apparatus but not into other similar positions on the same biological reaction apparatus). A barcode and/or an RFID tag can be associated with a wall of the container, for example, associated with an outer wall.
Various changes may be made without departing from the spirit and scope of the invention. For example, not all system functions need to be performed on a given tray. Thus, for example, a tray may be inserted into the apparatus for coverslipping only. Alternatively, the apparatus may include two or more de-paraffinizing/staining/solvent exchange station modules and/or two or more other modules in order to increase through-put. A feature of a particular embodiment is that additional station modules can be added vertically without increasing the footprint of the system. Other reagents may be utilized on the instrument to perform other tests, including those used for in situ hybridization (typically DNA/RNA probes), or immunohistochemistry (typically antibodies). In addition to microscope slides, tissue, DNA, RNA and protein arrays may also be accommodated with minimal or no modification of the slide trays. Yet other changes may be made in the invention without departing from the spirit and scope thereof, the scope of the invention being defined by the appended claims to be interpreted in light of the foregoing specification.
This application is a Continuation of U.S. patent application Ser. No. 16/399,592, filed Apr. 30, 2019 (U.S. Pat. No. 11,092,611), which is a Continuation of U.S. patent application Ser. No. 15/351,411, filed Nov. 14, 2016 (U.S. Pat. No. 10,302,665), which is a Continuation of U.S. patent application Ser. No. 14/082,092, filed Nov. 15, 2013 (U.S. Pat. No. 9,528,918), which is a Continuation of U.S. patent application Ser. No. 11/181,625, filed Jul. 13, 2005 (U.S. Pat. No. 8,663,991), which is a Divisional of U.S. patent application Ser. No. 11/116,676, filed Apr. 27, 2005 (U.S. Pat. No. 7,468,161), which is a Continuation-in-Part of U.S. patent application Ser. No. 10/414,804, filed Apr. 15, 2003 (U.S. Pat. No. 7,303,725), which claims the benefit of U.S. Provisional Patent Application No. 60/372,506, filed Apr. 15, 2002. The contents of these related applications and patents are incorporated by reference herein.
Number | Name | Date | Kind |
---|---|---|---|
3219416 | Natelson | Nov 1965 | A |
3574064 | Oinnings et al. | Apr 1971 | A |
3650437 | Oinnings et al. | Mar 1972 | A |
3665148 | Yasenchak et al. | May 1972 | A |
3695281 | Leon | Oct 1972 | A |
3853092 | Amos et al. | Dec 1974 | A |
3854703 | Gibbs et al. | Dec 1974 | A |
3979576 | Janson | Sep 1976 | A |
4013038 | Rogers et al. | Mar 1977 | A |
4043292 | Rogers et al. | Aug 1977 | A |
4058367 | Gilford | Nov 1977 | A |
4092952 | Wilkie et al. | Jun 1978 | A |
4245967 | Busselet | Jan 1981 | A |
RE30730 | Duff | Sep 1981 | E |
4286637 | Wilson | Sep 1981 | A |
4298571 | DiFulvio et al. | Nov 1981 | A |
4346056 | Sakurada | Aug 1982 | A |
4358470 | Rasmussen | Nov 1982 | A |
4384193 | Kledzik et al. | May 1983 | A |
4406547 | Aihara | Sep 1983 | A |
4413584 | DiMaggio | Nov 1983 | A |
4430299 | Horne | Feb 1984 | A |
4447395 | Englar et al. | May 1984 | A |
4453807 | Faulkner et al. | Jun 1984 | A |
4455280 | Shinohara et al. | Jun 1984 | A |
4484293 | Minucciani et al. | Nov 1984 | A |
4528159 | Liston | Jul 1985 | A |
4539855 | Jacobs | Sep 1985 | A |
4543236 | Von Gise | Sep 1985 | A |
4577514 | Bradley et al. | Mar 1986 | A |
4584275 | Okano et al. | Apr 1986 | A |
4629862 | Kitagawa et al. | Dec 1986 | A |
4643879 | Hanaway | Feb 1987 | A |
4647431 | Sekine et al. | Mar 1987 | A |
4648023 | Powell | Mar 1987 | A |
4659971 | Suzuki et al. | Apr 1987 | A |
4670974 | Antoszewksi et al. | Jun 1987 | A |
4676951 | Armes et al. | Jun 1987 | A |
4678752 | Thorne et al. | Jul 1987 | A |
4681741 | Hanaway | Jul 1987 | A |
4695430 | Coville et al. | Sep 1987 | A |
4708886 | Nelson | Nov 1987 | A |
4720463 | Farber et al. | Jan 1988 | A |
4727409 | Conner et al. | Feb 1988 | A |
4727494 | Ute | Feb 1988 | A |
4729661 | Bell | Mar 1988 | A |
4731335 | Brigati | Mar 1988 | A |
4731355 | Iwasaki et al. | Mar 1988 | A |
4738824 | Takeuchi | Apr 1988 | A |
4764342 | Kelln et al. | Aug 1988 | A |
4774055 | Wakatake et al. | Sep 1988 | A |
4777020 | Brigati | Oct 1988 | A |
4781891 | Galle et al. | Nov 1988 | A |
4795710 | Muszak et al. | Jan 1989 | A |
4798706 | Brigati | Jan 1989 | A |
4801431 | Cuomo et al. | Jan 1989 | A |
4805469 | Commarmot | Feb 1989 | A |
4807152 | Lane et al. | Feb 1989 | A |
4815978 | Mazza et al. | Mar 1989 | A |
4835711 | Hutchins et al. | May 1989 | A |
4837159 | Yamada | Jun 1989 | A |
4843566 | Gordon et al. | Jun 1989 | A |
4844868 | Rokugawa | Jul 1989 | A |
4847208 | Bogen | Jul 1989 | A |
4852001 | Tsushima et al. | Jul 1989 | A |
4855109 | Muraishi et al. | Aug 1989 | A |
4857272 | Sugaya | Aug 1989 | A |
4858155 | Okawa et al. | Aug 1989 | A |
4865986 | Coy et al. | Sep 1989 | A |
4895706 | Root et al. | Jan 1990 | A |
4896269 | Tong | Jan 1990 | A |
4902481 | Clark et al. | Feb 1990 | A |
4911098 | Tabata | Mar 1990 | A |
4911915 | Fredenburgh | Mar 1990 | A |
4919887 | Wakatake | Apr 1990 | A |
4928540 | Kido et al. | May 1990 | A |
4933146 | Meyer et al. | Jun 1990 | A |
4935875 | Shah et al. | Jun 1990 | A |
4961906 | Andersen et al. | Oct 1990 | A |
4964544 | Hanna et al. | Oct 1990 | A |
4965049 | Lillig et al. | Oct 1990 | A |
4971913 | Manabe et al. | Nov 1990 | A |
4975250 | Mordecki | Dec 1990 | A |
4979093 | Laine et al. | Dec 1990 | A |
4979128 | Seki et al. | Dec 1990 | A |
4985206 | Bowman et al. | Jan 1991 | A |
5002736 | Babbitt et al. | Mar 1991 | A |
5023187 | Koebler et al. | Jun 1991 | A |
5030418 | Miyata | Jul 1991 | A |
5035866 | Wannlund | Jul 1991 | A |
5040123 | Barber et al. | Aug 1991 | A |
5051238 | Umetsu et al. | Sep 1991 | A |
5073504 | Bogen | Dec 1991 | A |
5075079 | Kerr et al. | Dec 1991 | A |
5089229 | Heidt et al. | Feb 1992 | A |
5093557 | Lok et al. | Mar 1992 | A |
5096670 | Harris et al. | Mar 1992 | A |
5104621 | Pfost et al. | Apr 1992 | A |
5105066 | Houdy et al. | Apr 1992 | A |
5116496 | Scott | May 1992 | A |
5122342 | McCulloch et al. | Jun 1992 | A |
5122959 | Nathanson et al. | Jun 1992 | A |
5148370 | Litt et al. | Sep 1992 | A |
5154889 | Muraishi | Oct 1992 | A |
5168453 | Nomaru et al. | Dec 1992 | A |
5180606 | Stokes et al. | Jan 1993 | A |
5181259 | Rorvig | Jan 1993 | A |
5207987 | Kureshy et al. | May 1993 | A |
5209903 | Kanamori et al. | May 1993 | A |
5218645 | Bacus | Jun 1993 | A |
5229074 | Heath et al. | Jul 1993 | A |
5231029 | Wootton et al. | Jul 1993 | A |
5232664 | Krawzak et al. | Aug 1993 | A |
5232665 | Burkovich et al. | Aug 1993 | A |
5233533 | Edstrom et al. | Aug 1993 | A |
5246665 | Tyranski et al. | Sep 1993 | A |
5266272 | Griner et al. | Nov 1993 | A |
5273905 | Muller et al. | Dec 1993 | A |
5280156 | Niori et al. | Jan 1994 | A |
5282149 | Grandone et al. | Jan 1994 | A |
5304347 | Mann et al. | Apr 1994 | A |
5311426 | Donohue et al. | May 1994 | A |
5314825 | Weyrauch et al. | May 1994 | A |
5316452 | Bogen et al. | May 1994 | A |
5316726 | Babson et al. | May 1994 | A |
5332549 | MacIndoe, Jr. | Jul 1994 | A |
5334353 | Blattner | Aug 1994 | A |
5352612 | Huber et al. | Oct 1994 | A |
5355439 | Bernstein et al. | Oct 1994 | A |
5355695 | Kawaguchi | Oct 1994 | A |
5356595 | Kanamori et al. | Oct 1994 | A |
5356814 | Carrico, Jr. et al. | Oct 1994 | A |
5358691 | Clark et al. | Oct 1994 | A |
5376313 | Kanewske, III et al. | Dec 1994 | A |
5402350 | Kline | Mar 1995 | A |
5424036 | Ushikubo | Jun 1995 | A |
5425918 | Healey et al. | Jun 1995 | A |
5428470 | Labriola, II | Jun 1995 | A |
5431309 | Ophardt | Jul 1995 | A |
5439645 | Saralegui et al. | Aug 1995 | A |
5439649 | Tseung et al. | Aug 1995 | A |
5446652 | Peterson et al. | Aug 1995 | A |
5475610 | Atwood et al. | Dec 1995 | A |
5479581 | Kleinschnitz | Dec 1995 | A |
5492837 | Naser-Kolahzadeh et al. | Feb 1996 | A |
5496518 | Arai et al. | Mar 1996 | A |
5512248 | Van | Apr 1996 | A |
5523056 | Miller | Jun 1996 | A |
5525302 | Astle | Jun 1996 | A |
5525515 | Blattner | Jun 1996 | A |
5573727 | Keefe | Nov 1996 | A |
5575976 | Choperena et al. | Nov 1996 | A |
5576215 | Burns et al. | Nov 1996 | A |
5578455 | Tosa et al. | Nov 1996 | A |
5595707 | Copeland et al. | Jan 1997 | A |
5601141 | Gordon et al. | Feb 1997 | A |
5614376 | Copley et al. | Mar 1997 | A |
5629201 | Nugteren et al. | May 1997 | A |
5639665 | Arai et al. | Jun 1997 | A |
5645114 | Bogen et al. | Jul 1997 | A |
5645800 | Masterson et al. | Jul 1997 | A |
5646046 | Fischer et al. | Jul 1997 | A |
5646049 | Tayi | Jul 1997 | A |
5650327 | Copeland et al. | Jul 1997 | A |
5654199 | Copeland et al. | Aug 1997 | A |
5654200 | Copeland et al. | Aug 1997 | A |
5656493 | Mullis et al. | Aug 1997 | A |
5672512 | Shaw | Sep 1997 | A |
5674454 | Karl et al. | Oct 1997 | A |
5675715 | Bernstein et al. | Oct 1997 | A |
5690892 | Babler et al. | Nov 1997 | A |
5695718 | Imai et al. | Dec 1997 | A |
5696887 | Bernstein et al. | Dec 1997 | A |
5700346 | Edwards | Dec 1997 | A |
5736105 | Astle | Apr 1998 | A |
5737498 | Murray | Apr 1998 | A |
5737499 | Bernstein et al. | Apr 1998 | A |
5819842 | Potter et al. | Oct 1998 | A |
5839091 | Rhett et al. | Nov 1998 | A |
5854075 | Levine et al. | Dec 1998 | A |
5861094 | Goehde | Jan 1999 | A |
5869006 | Fanning et al. | Feb 1999 | A |
5871696 | Roberts | Feb 1999 | A |
5875286 | Bernstein et al. | Feb 1999 | A |
5895628 | Heid et al. | Apr 1999 | A |
5909674 | Schaffer et al. | Jun 1999 | A |
5917675 | Yang et al. | Jun 1999 | A |
5930461 | Bernstein et al. | Jul 1999 | A |
5947167 | Bogen et al. | Sep 1999 | A |
5948349 | Beurotte et al. | Sep 1999 | A |
5948359 | Kalra | Sep 1999 | A |
5958341 | Chu | Sep 1999 | A |
5975740 | Lin et al. | Nov 1999 | A |
5985214 | Stylli | Nov 1999 | A |
5985669 | Palander | Nov 1999 | A |
5985672 | Kegelman et al. | Nov 1999 | A |
6004512 | Titcomb et al. | Dec 1999 | A |
6017495 | Ljungmann | Jan 2000 | A |
6054099 | Levy | Apr 2000 | A |
6068393 | Hutchins et al. | May 2000 | A |
6076583 | Edwards | Jun 2000 | A |
6080363 | Takahashi et al. | Jun 2000 | A |
6093574 | Druyor-Sanchez et al. | Jul 2000 | A |
6096271 | Bogen et al. | Aug 2000 | A |
6110425 | Gao et al. | Aug 2000 | A |
6136270 | Maes et al. | Oct 2000 | A |
6180060 | Green et al. | Jan 2001 | B1 |
6180061 | Bogen et al. | Jan 2001 | B1 |
6183645 | DeWitt | Feb 2001 | B1 |
6183693 | Bogen et al. | Feb 2001 | B1 |
6193933 | Sasaki et al. | Feb 2001 | B1 |
6258322 | Meikle | Jul 2001 | B1 |
6284543 | Alvarez | Sep 2001 | B1 |
6296764 | Guirguis et al. | Oct 2001 | B1 |
6296809 | Richards et al. | Oct 2001 | B1 |
6349264 | Rhett et al. | Feb 2002 | B1 |
6352861 | Copeland et al. | Mar 2002 | B1 |
6368067 | Stutz | Apr 2002 | B1 |
6372144 | Vassarotti | Apr 2002 | B1 |
6387326 | Edwards et al. | May 2002 | B1 |
6395554 | Regan et al. | May 2002 | B1 |
6436348 | Ljungmann et al. | Aug 2002 | B1 |
6451551 | Zhan et al. | Sep 2002 | B1 |
6471958 | Dimitrijevich et al. | Oct 2002 | B2 |
6472217 | Richards et al. | Oct 2002 | B1 |
6495106 | Kalra | Dec 2002 | B1 |
6537818 | Richards et al. | Mar 2003 | B2 |
6585936 | Shah | Jul 2003 | B1 |
6594537 | Bernstein et al. | Jul 2003 | B1 |
6626224 | Ljungmann | Sep 2003 | B1 |
6632598 | Zhang et al. | Oct 2003 | B1 |
6635225 | Thiem et al. | Oct 2003 | B1 |
6649128 | Meyer et al. | Nov 2003 | B1 |
6685884 | Stylli et al. | Feb 2004 | B2 |
6703247 | Chu | Mar 2004 | B1 |
6746851 | Tseung et al. | Jun 2004 | B1 |
6759011 | Richards et al. | Jul 2004 | B1 |
6821072 | Thiem et al. | Nov 2004 | B2 |
6827900 | Thiem et al. | Dec 2004 | B2 |
6827901 | Copeland et al. | Dec 2004 | B2 |
6881579 | Hilson et al. | Apr 2005 | B2 |
6887428 | Wernz et al. | May 2005 | B2 |
6979425 | Ganz | Dec 2005 | B1 |
6998094 | Haslam et al. | Feb 2006 | B2 |
6998270 | Tseung et al. | Feb 2006 | B2 |
7025933 | Ganz | Apr 2006 | B2 |
7153474 | Thiem | Dec 2006 | B2 |
7262022 | Chu | Aug 2007 | B2 |
7270785 | Lemme et al. | Sep 2007 | B1 |
7271006 | Reinhardt et al. | Sep 2007 | B2 |
7273591 | Sellers et al. | Sep 2007 | B2 |
7303725 | Reinhardt et al. | Dec 2007 | B2 |
7314595 | Honkanen et al. | Jan 2008 | B2 |
7368081 | Thiem | May 2008 | B2 |
7435383 | Tseung et al. | Oct 2008 | B2 |
7468161 | Reinhardt et al. | Dec 2008 | B2 |
7501283 | Hersch et al. | Mar 2009 | B2 |
7553672 | Bogen et al. | Jun 2009 | B2 |
7584019 | Feingold et al. | Sep 2009 | B2 |
7744817 | Bui | Jun 2010 | B2 |
7860727 | Showalter et al. | Dec 2010 | B2 |
7964141 | Heid | Jun 2011 | B2 |
8048373 | Reinhardt et al. | Nov 2011 | B2 |
8288121 | Kram et al. | Oct 2012 | B2 |
8454908 | Lapen | Jun 2013 | B2 |
8622681 | Rippl | Jan 2014 | B2 |
8663991 | Reinhardt et al. | Mar 2014 | B2 |
8719053 | Showalter et al. | May 2014 | B2 |
9528918 | Reinhardt et al. | Dec 2016 | B2 |
9891147 | Lapen | Feb 2018 | B2 |
10302665 | Reinhardt et al. | May 2019 | B2 |
10900982 | Reinhardt et al. | Jan 2021 | B2 |
11092611 | Reinhardt et al. | Aug 2021 | B2 |
20010004449 | Suzuki et al. | Jun 2001 | A1 |
20010016358 | Osawa et al. | Aug 2001 | A1 |
20010019702 | Watari et al. | Sep 2001 | A1 |
20010019703 | Thiem et al. | Sep 2001 | A1 |
20010055545 | Takii et al. | Dec 2001 | A1 |
20020018733 | Kapplein et al. | Feb 2002 | A1 |
20020037239 | Komatsu | Mar 2002 | A1 |
20020054830 | Bogen et al. | May 2002 | A1 |
20020057992 | Eckert et al. | May 2002 | A1 |
20020064482 | Tisone et al. | May 2002 | A1 |
20020110494 | Lemme et al. | Aug 2002 | A1 |
20020116132 | Rhett et al. | Aug 2002 | A1 |
20020182115 | Aghassi et al. | Dec 2002 | A1 |
20030026732 | Gordon et al. | Feb 2003 | A1 |
20030032191 | Hilson | Feb 2003 | A1 |
20030047863 | Lang et al. | Mar 2003 | A1 |
20030049104 | Thiem et al. | Mar 2003 | A1 |
20030087292 | Chen et al. | May 2003 | A1 |
20030092186 | Pressman et al. | May 2003 | A1 |
20030099580 | Pressman et al. | May 2003 | A1 |
20030138353 | Bargoot | Jul 2003 | A1 |
20030161761 | Williams et al. | Aug 2003 | A1 |
20030203493 | Lemme et al. | Oct 2003 | A1 |
20030211630 | Richards et al. | Nov 2003 | A1 |
20030215357 | Malterer et al. | Nov 2003 | A1 |
20030215936 | Kallioniemi et al. | Nov 2003 | A1 |
20030231987 | Carmack et al. | Dec 2003 | A1 |
20040001390 | Manaka | Jan 2004 | A1 |
20040002163 | Reinhardt et al. | Jan 2004 | A1 |
20040009098 | Torre-Bueno | Jan 2004 | A1 |
20040023371 | Fawcett | Feb 2004 | A1 |
20040038408 | Abbott et al. | Feb 2004 | A1 |
20040052685 | Richards et al. | Mar 2004 | A1 |
20040082058 | Schleifer et al. | Apr 2004 | A1 |
20040092024 | Reinhardt et al. | May 2004 | A1 |
20040121485 | Hopkins et al. | Jun 2004 | A1 |
20040136868 | Bevirt et al. | Jul 2004 | A1 |
20040197230 | Lemme et al. | Oct 2004 | A1 |
20050042137 | Petersen et al. | Feb 2005 | A1 |
20050047971 | Clements et al. | Mar 2005 | A1 |
20050053526 | Angros | Mar 2005 | A1 |
20050089444 | Justin et al. | Apr 2005 | A1 |
20050089949 | Baer et al. | Apr 2005 | A1 |
20050118670 | Lihl et al. | Jun 2005 | A1 |
20050135971 | Rich | Jun 2005 | A1 |
20050153453 | Copeland et al. | Jul 2005 | A1 |
20050164374 | Kram | Jul 2005 | A1 |
20050186114 | Reinhardt et al. | Aug 2005 | A1 |
20050238534 | Chu | Oct 2005 | A1 |
20050250211 | Reinhardt et al. | Nov 2005 | A1 |
20050270642 | McLellan et al. | Dec 2005 | A1 |
20060019302 | Lemme et al. | Jan 2006 | A1 |
20060035369 | Gauer et al. | Feb 2006 | A1 |
20060051253 | Gausepohl | Mar 2006 | A1 |
20060088928 | Sweet et al. | Apr 2006 | A1 |
20060105462 | Sellek-Prince | May 2006 | A1 |
20060120621 | Larkin et al. | Jun 2006 | A1 |
20060120921 | Elliot et al. | Jun 2006 | A1 |
20060120925 | Takayama et al. | Jun 2006 | A1 |
20060127276 | Ljungmann et al. | Jun 2006 | A1 |
20060134732 | Kram et al. | Jun 2006 | A1 |
20060148063 | Fauzzi et al. | Jul 2006 | A1 |
20060166371 | Testa et al. | Jul 2006 | A1 |
20060231023 | Angros | Oct 2006 | A1 |
20080050511 | Sellek-Prince | Feb 2008 | A1 |
20080318305 | Angros | Dec 2008 | A1 |
20100031757 | Hoyer | Feb 2010 | A1 |
20110217731 | Burgart et al. | Sep 2011 | A1 |
20130052331 | Kram et al. | Feb 2013 | A1 |
20130203100 | Otter et al. | Aug 2013 | A1 |
20150071833 | Kram et al. | Mar 2015 | A1 |
20190257846 | Reinhardt et al. | Aug 2019 | A1 |
20190257847 | Reinhardt et al. | Aug 2019 | A1 |
Number | Date | Country |
---|---|---|
2005203557 | Aug 2006 | AU |
2003224987 | Sep 2009 | AU |
2321823 | Sep 1999 | CA |
2482441 | Oct 2003 | CA |
240134 | Oct 1987 | EP |
517835 | Dec 1992 | EP |
600939 | Jun 1994 | EP |
517835 | Feb 1996 | EP |
722363 | Jul 1996 | EP |
722363 | Apr 1999 | EP |
600939 | Oct 1999 | EP |
1052497 | Nov 2000 | EP |
1477838 | Nov 2004 | EP |
1890127 | Feb 2008 | EP |
2239167 | Feb 1975 | FR |
2528122 | Dec 1983 | FR |
2143205 | Feb 1985 | GB |
2216259 | Oct 1989 | GB |
55014157 | Jan 1980 | JP |
55107957 | Aug 1980 | JP |
61219847 | Sep 1986 | JP |
63208761 | Aug 1988 | JP |
4356845 | Dec 1992 | JP |
5504627 | Jul 1993 | JP |
2009503304 | Mar 1997 | JP |
2001242175 | Sep 2001 | JP |
2001516869 | Oct 2001 | JP |
2002511600 | Apr 2002 | JP |
2002267642 | Sep 2002 | JP |
2002267942 | Sep 2002 | JP |
2003344242 | Dec 2003 | JP |
2004506228 | Feb 2004 | JP |
2013092532 | May 2013 | JP |
1987000086 | Jan 1987 | WO |
1988002865 | Apr 1988 | WO |
1991013335 | Sep 1991 | WO |
1992001919 | Feb 1992 | WO |
1992019952 | Nov 1992 | WO |
1993023732 | Nov 1993 | WO |
1995010035 | Apr 1995 | WO |
1995024498 | Sep 1995 | WO |
1999009390 | Feb 1999 | WO |
1999044032 | Sep 1999 | WO |
1999053357 | Oct 1999 | WO |
2000014534 | Mar 2000 | WO |
2000062035 | Oct 2000 | WO |
2001051909 | Jul 2001 | WO |
2001073399 | Oct 2001 | WO |
2002012857 | Feb 2002 | WO |
2002074525 | Sep 2002 | WO |
2003045560 | Jun 2003 | WO |
2003052386 | Jun 2003 | WO |
2003089140 | Oct 2003 | WO |
2003091710 | Nov 2003 | WO |
2003106157 | Dec 2003 | WO |
2004001390 | Dec 2003 | WO |
2004008106 | Jan 2004 | WO |
2004074845 | Sep 2004 | WO |
2005031312 | Apr 2005 | WO |
2006073910 | Jul 2006 | WO |
Entry |
---|
Lindsey, J. S. et al., “Robotic Work Station for Microscale Synthetic Chemistry: On-Line Absorption Spectroscopy, Quantitative Automated Thin-Layer Chromatography, and Multiple Reactions in Parallel,” Review of Scientific Instruments, vol. 59, No. 6, Jun. 1988, pp. 940-950. |
Montone, K. T. et al., “Anatomic Viral Detection Is Automated: The Application of a Robotic Molecular Pathology System for the Detection of DNA Viruses in Anatomic Patholgy Substrates, Using Immunocytochemical and Nucleic Acid Hybridization Techniques,” The Yale Journal of Biology and Medicine, vol. 62, 1989, pp. 141-158. |
“Advanta CV/AS,” Article from Vision Instruments, Date: Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 2 pgs. |
“Capillary Action Slide Stainers for Histology and Cytology,” Article from Fisher Scientific, Date Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 4 pgs. |
“Coverslips and Stainers”, Hacker Instruments and Industries, Inc., 3 pages, [retrieved on Apr. 18, 2001], Retrieved from the Internet <URL: http://hackerinstruments.com/coverslippers.htm>. |
“DAKO Autostainer Features and Specifications,” DAKO Corporation, 3 pages, [retrieved on Dec. 7, 2000], Retrieved from the Internet <URL: http://www.dakousa.com>. |
“I 6000,” Article from BioGenex, 2000, 4 pages. |
“Laboratory Equipment 1998 and 1999”, Article from Shandon, Inc., pp. 37-51. |
“Leica Auto Stainer XL,” Article from Leica, Date: Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 4 pgs. |
“Robot-Stainer HMS 760, Automatic Slide Stainer for Routine Histology and Cytology Applications,” Article from Microm Histology Products, Date: Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 4 pgs. |
“Sakura Tissue-Tek DRS 2000 Slide Stainer”, Article from Sakura Finetek U.S.A., Inc., 1998, 1 page. |
“ST 5050 Zymed's Sensible IHC Automated Staining Solution”, article from Zymed Laboratories, 2 pages. |
“The New Protocol in Staining Technology,” Article from Fisher Healthcare, Date: Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 5 pgs. |
“Tissue-Stainer TST 40,” Article from Medite, Date: Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 2 pgs. |
“Tissue-Tek DRS 2000 Automatic Multiple Slide Stainer: Multiple with Double Quality,” Article from Sakura Fintek Europe B.V., 1998, 4 pages. |
“Tissue-Tek DRS 2000 Slide Stainer: Computer-Assisted Flexibility for Unmatched Productivity,” Article from Sakura Finetek, U.S.A., Inc., 1998, 4 pages. |
“TST Stainer Trio,” Article from Mopec, Date: Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 7 pgs. |
“Varistain 24-4: Flexible, Efficient Automatic Slide Stainer,” article from Shandon, Inc., 1991, 8 pages. |
“Varistain 24-4K: High Throughput Continuous Slide Stainer,” article from Shandon, Inc., 1991, 2 pages. |
“Varistain XY Multi-Program Robotic Slide Stainer,” article from Shandon, Inc., 1991, 8 pages. |
Bartusch, M. et al., “Scheduling Project Networks with Resource Constraints and Time Windows”, Annals of Operations Research, vol. 16, 1988, pp. 201-240. |
Brigati, D. J. et al., “Immunocytochemistry is Automated: Development of a Robotic Workstation Based Upon the Capillary Action Principle”, The Journal of Histotechnology, vol. 11, No. 3, Sep. 1998, pp. 165-183. |
Conference Proceedings Presented at the 2000 National Society for Histotechnology Convention, “An Automated In Situ Hybridization System with High Throughput Capabilities,” Biogenex, 2000, 2 pages. |
Critchlow, A. J., “Introduction to Robotics”, MacMillan Publishing Co., New York, 1985, pp. 37-56, 151-213. |
Driscoll, R. C. et al., “II Analytical Systems: Discrete Automated Chemistry System with Tableted Reagents,” Clinical Chemistry, vol. 29, No. 9, 1983, pp. 1609-1615. |
Flore, M. et al., “The Abbott IMx Automated Benchtop Immunochemistry Analyzer System”, Clinical Chemistry, vol. 34, No. 9, 1988, pp. 1726-1732. |
Fouda, H. G. et al., “Robotics for the bioanalytical laboratory: A flexible system for the analysis of drugs in biological fluids”, Trac Trends in Analytical Chemistry, 1987, 10 pages. |
Hamacher, V. C. et al., “Computer Organization”, 2nd Edition, McGraw-Hill Book Company, New York, pp. 1-14. |
Hayes, F. et al., “A Guide to GUIs”, Byte, Jul. 1989, pp. 250-257. |
Innis, M. A. et al., “DNA sequencing with Thermus aquaticus DNA polymerase and direct sequencing of polymerase chain reaction-amplified DNA”, Proceedings of the National Academy of Sciences USA, vol. 85, Dec. 1988, pp. 9436-9440. |
International Searching Authority, International Search Report for PCT/US2003/11651, dated Jul. 30, 2003, Applicant: Ventana Medical Systems, Inc., 2 pages. |
Isenhour, T. L. et al., “Intelligent Robots—The Next Step in Laboratory Automation,” Analytical Chemistry, vol. 61, No. 13, Jul. 1989, pp. 805-814. |
Isenhour, T. L. et al., “Laboratory Robotics and Artificial Intelligence”, Clinical Chemistry, vol. 36, No. 9, 1990, pp. 1561-1566. |
Isenhour, T. L. et al., “TORTS: An Expert System for Temporal Optimization of Robotic Procedures”, Journal of Chemical Information and Computer Sciences, vol. 28, No. 4, 1988, pp. 215-221. |
Isenhour, T. L., “Robotics in the Laboratory”, Journal of Chemical Information and Computer Sciences, vol. 25, No. 3, 1985, pp. 292-295. |
Kawaba, S. et al., “Robot Task Planning System Based on Product Modeling”, IEEE, 1985, pp. 471-476. |
Leica ST 4040 and Leica Autostainer XL, description, Date: Unknown (for purposes of examination date is assumed to be prior to filing date of Apr. 15, 2002), 1 page. |
Longnecker, D. S., “A Program for Automated Hematoxylin and Eosin Staining”, Technical Bulletin of the Registry of Medical Technologists, vol. 36, No. 1, 1966, p. 19. |
Mawhinney, W. H. B. et al., “Automated immunochemistry”, Journal of Clinical Pathology, vol. 43, 1990, pp. 591-596. |
McCahon, C. S. et al., “Job Sequencing with Fuzzy Processing Times”, Computers & Mathematics with Applications, vol. 19, No. 7, 1990, pp. 31-41. |
Mueller N. J. et al., “Concurrent HPLC Analyses of Carbohydrate Distribution and 5-(Hydroxymethyl)-2-Furaldehyde Using Robotics”, Journal of Chromatographic Science, vol. 25, 1987, pp. 198-201. |
Okino, N. et al., “Robot Simulator in Tips/Geometric Simulator”, Robotics and Computer Integrated Manufacturing, vol. 3, No. 4, 1987, pp. 429-437. |
Plakhtin, D. L., “Use of Automatic Devices for Histological Processing and Staining of the Tissues and Certain Characteristics of Preparation of Histological Specimens”, Arkh Patol, vol. 38, No. 11, 1976, pp. 76-77, Abstract Only. |
Saiki, R. K. et al., “Enzymatic Amplification of β-Globin Genomic Sequences and Restriction Site Analysis for Diagnosis of Sickle Cell Anemia”, Science, vol. 230, Dec. 1985, pp. 1350-1354. |
Sjolund, P. et al., “Robot Task Planning: Programming Using Interactive Computer Graphics,” Apr. 1983, pp. 7-122-7-135. |
Solomon, M. M. et al., “Time Window Constrained Routing and Scheduling Problems”, Transportation Science, vol. 22, No. 1, Feb. 1988, pp. 1-13. |
Stark, E. et al., “An Automated Device for Immunocytochemistry”, Journal of Immunological Methods, vol. 107, 1988, pp. 89-92. |
Stelzner, M. et al., “The SimKit System: Knowledge-Based Simulation and Modeling Tools in Kee”, An Intellicorp Technical Article, 1987, 22 pages. |
Stress, W. P. et al., “Automation of APAAP Immunocytochemical Technique”, Journal of Clinical Pathology, vol. 42, 1989, pp. 106-112. |
Unger, E. R. et al., “Colorimetric In-Situ Hybridization in Clinical Virology: Development of Automated Technology”, Current Topics in Microbiology and Immunology, vol. 143, 1989, pp. 21-31. |
Unger, E. R. et al., “Viral Diagnosis by In Situ Hybridization: Description of a Rapid Simplified CoIometric Method”, The American Journal of Surgical Pathology, vol. 10, No. 1, 1986, pp. 1-8. |
Viglierchio, D.R., et al., “Automatic Solvent Exchanger,” Transactions of the American Microscopical Society 84, Department of Nematology, University of California, Davis, 1965, pp. 284-293. |
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