Recent research initiatives have spawned an increased effort to streamline the various processes used to perform Life Sciences research. The complexity of biological organisms has necessitated the development of a range of laboratory procedures to manipulate biological materials. There is a particular need to isolate various substances such as nucleic acids, proteins, cellular metabolites, carbohydrates and lipids from such biological materials in order to perform the analytical processes used to define and interpret living systems. At the same time, technological advancements have begun to make it possible to analyze biological organisms in a more comprehensive, holistic manner. High throughput analytical technologies have led to advancements in genomics, proteomics, metabolomics and systems biology. Nevertheless, while there has been substantial advancement in developing efficient high throughput analytical processes, the fundamental requirement to prepare biological and biochemical substances for analysis remains a rate limiting step to full implementation of these analytical methods.
There are various methods for preparing biological and biochemical substances and these methods generally include a series of steps in which a substance of interest is processed, for example, by sequentially collecting material, such as by adsorption, sedimentation, centrifugation or filtration; modifying the starting substance, such as by treatment with chaotropic agents, or lysing cellular materials; separating a selected sub-fraction of the material collected, for example, by performing gel chromatography, filtration, or selective adsorption to a binding matrix; further separating sub-fractions, such as by washing with liquids like appropriate wash buffers, or by selective elution of sub-fractions from a gel or binding matrix, and releasing, eluting or collecting the processed material to yield a desired substance, for example, a substantially purified nucleic acid, protein, carbohydrate, or lipid molecule. Historically, all of these methods have necessarily required multiple transfers of the material being processed from one container to others, in series as the processing procedure is carried out.
Specific substances that must be prepared from biological materials to analyze biological organisms include: single and double stranded DNA molecules from bacteriophages; bacterial plasmids; fungal plasmids such as yeast plasmids; Bacterial Artificial Chromosomes (BAC's); viral nucleic acids, genomic DNA from a variety of cell types such as genomic DNA from nucleated blood cells; protein molecules; antibody molecules; RNA molecules; carbohydrate molecules; lipid molecules; and cell metabolites.
In addition, it is also important to be able to process biochemical samples generated by in vitro manipulations of various macromolecules in order to conduct further biochemical manipulation or analysis. Examples of such processes include: nucleic acid template preparation for biochemical manipulations such as PCR or DNA sequencing; the clean-up of biochemical reaction products, such as DNA thermocycle sequencing products; the clean-up of PCR reaction products for further manipulation and/or analysis; the preparation of biochemically modified or processed protein molecules for further modification or analysis, such as preparation of protein fragments for analysis by MALDI-TOF mass spectrometry; and the preparation of labeled nucleic acid samples, such as cDNA labeled with fluorescent dyes for expression analysis with gene chips or spotted arrays.
Thus, there is a need for broadly applicable technology that can be easily adapted to perform a variety of sample processing procedures that share common process elements.
A specific case where there is a need to improve the efficiency of sample preparation processes is in the preparation of DNA template molecules for analysis by DNA sequencing. Standard methods for purifying plasmid templates for sequencing have been developed by incremental modification of a few traditional procedures that necessarily require a significant number of steps and the transfer of liquid samples from container to container. For example, current protocols for purifying nucleic acid samples for sequencing include an initial centrifugation step, which is used to collect and concentrate cultured bacterial cells that contain cloned DNA molecules so that the cloned molecules can be purified. Because this step must be accomplished without the loss of the sample, the centrifugation must be performed in a sample container that is completely sealed at the bottom.
Many of these protocols also include a filtration step, wherein the sample substance containing the nucleic acid and waste products is passed through a filtering means. The filter material selectively binds to the target nucleic acid, while allowing the liquid and waste products to flow through. Because it is necessary to remove the waste products and liquid after filtration, this step must be performed in a sample container which already includes an opening below the filtering means. Examples of such containers are shown in U.S. Pat. No. 4,683,058 (1987, Lyman et al.), U.S. Pat. No. 5,264,184 (1993, Aysta et al.), and U.S. Pat. No. 5,910,246 (1999, Walter et al.); the teachings of which are incorporated by reference.
Since the container requirements for these two steps are incompatible, the sample must be transferred from the closed container (used for centrifugation) to the container which includes the opening (used for the filtration step), which adds a step to the overall process. Furthermore, the closed containers (usually plastic test tubes) are discarded after the transfer. If the same container or test tube could be used for both the centrifugation and filtration steps, the time consuming transfer step could be eliminated, and the amount of solid waste generated could be reduced. Therefore, there is a long felt need for a method and apparatus for processing substances in a single container.
The sequencing of DNA has long been relegated to the controlled environment of the research laboratory. In order to ensure high quality data, current laboratory protocols implement many precise, manual operations which could only be performed by skilled technicians. Although numerous mechanical devices exist to perform some of these individual operations, the overall number of operations remains large, and each of these devices still requires skilled supervision. Furthermore, each additional step in the process is a potential source of error. A particularly time consuming part of the sequencing process is the isolation and purification of DNA templates from the bacterial cultures in which the DNA is cloned. Many existing methods for DNA template preparation have been adapted to the standard 96-well format, in which samples are batch processed in trays or plates, each containing 96 tubes or sample wells. One such method is disclosed in Anderson et al., Method for 96-well M13 DNA Template Preparations for Large-Scale Sequencing, BioTechniques (June 1996). Another example of such a method is disclosed in QIAprep 96 M13 Protocol, QIAprep M13 Handbook (2/99) from Qiagen Incorporated. These references are herein incorporated by reference.
Recent research initiatives have created great demand for large-scale, high-speed techniques for sequencing and mapping genetic material. Although several integrated machines have been developed which automate some or all of the template preparation process, these machines usually duplicate the manual operations of the previous methods without seeking to eliminate or consolidate steps. Furthermore, many of these methods require the use of expensive and highly specialized sample containers, which essentially have no other uses except as disclosed. Methods of this type are disclosed in U.S. Pat. No. 5,610,074 (Beritashvili et al., 1997) and U.S. Pat. No. 5,863,801 (Southgate et al., 1999), incorporated herein by reference. Thus, there is long felt need for a method or apparatus for processing substances in a single container.
An example of at least one such method and apparatus is seen in U.S. patent application Ser. No. 10/641,378 (filed Oct. 13, 2003, claiming priority to commonly-assigned U.S. patent application Ser. No. 09\658,017, which was filed Sep. 12, 2000, which was, in turn, a continuation-in-part of U.S. application Ser. No. 09/532,599, filed Mar. 22, 2000, and also commonly-assigned). Each of the preceding commonly-assigned applications is incorporated herein by reference.
Polynucleotides come in many forms and a number of alternative forms have been manipulated by recombinant DNA techniques to develop the common tools used to perform contemporary molecular biology research. For example, a “plasmid” is an extrachromosomal, autonomously replicating DNA molecule (also a polynucleotide) commonly employed in genetic research to carry out various manipulations of DNA polynucleotides. In a common use, DNA fragments cloned into plasmid molecules are used as a template for “DNA sequencing” to determine the exact series of bases (A, C, G or T mononucleotides) in a particular DNA fragment. The plasmid is replicated by host cells (e.g., bacterial cells). A virus, like a plasmid, is a polynucleotide molecule, but it can also infect host cells. The term “phage” is used to describe a group of bacterial viruses (“phage” means “eater” because these viruses were first observed as blank areas on carpets of bacterial cells where these holes in the bacterial growth appeared to have been eaten), and a “vector” is an engineered form of a polynucleotide capable of carrying another polynucleotide insert. “Cosmids,” are modified replicons that contain viral sequences derived from bacteriophage lambda that direct DNA replication but do not contain many viral structural genes such as coat proteins. Cosmids are engineered to carry relatively large polynucleotides inserts, 20-40 kb in length, and can be packaged in vitro into a viral coat protein. They can infect a cell and be propagated in vivo. “Phosmids,” are like cosmids, and contain sequences derived form both phagemid and cosmid vectors, thus combining functional properties of both of these systems. There are additional forms of polynucleotides (e.g., BACs or bacterial artificial chromosomes, PAC's, YAC's and others, each designed to perform alternative useful genetic manipulations).
A plasmid is an epigenetic element; it is not part of the host chromosomal DNA molecule. A large number of naturally occurring plasmid molecules have been isolated and analyzed, and a number of them have been modified to produce useful vectors for genetic manipulations including, but not limited to: cloning individual genes; facilitation of manipulation of polynucleotide sequences such as site specific mutagenesis; expression of recombinant proteins; and amplification of appropriate amounts of desired polynucleotide molecules for probes or genetic analysis. Others will occur to those of skill in the art.
Historically, plasmids were discovered in cells, and it was found that they could be separated from the cell, and engineered for a variety of purposes. When handled appropriately, plasmid DNA's are quite stable under typical laboratory conditions, so they can be prepared and stored easily and kept available for experimentation as needed. Furthermore, isolated plasmids can be re-introduced into alternative host cells by the process of transformation. Transformed bacteria are commonly used to prepare quantities of plasmid DNA for biochemical manipulation. This is accomplished by growing suitable volumes of plasmid containing bacteria in culture and then performing a plasmid purification process to isolate purified plasmid DNA
In traditional methods of preparation of cloned polynucleotides such as DNA fragments inserted into plasmid vectors, the first step used to isolate clones containing a single specific DNA insert is to spread a diluted mixture of a population of transformed bacteria onto an agar culture media in a petri plate. Bacteria are spread on the agar medium in numbers such that each individual cell will give rise to a distinct, isolated colony of identical cells that can be readily identified and subcultured to prepare a sufficient quantity of plasmid material. In some such processes, a toothpick is contacted with a colony of bacteria that have been grown in a petri dish in which there are multiple colonies of bacteria (each having a particular plasmid associated with the colony). The toothpick is then dropped in a well in a growth vessel or “plate” with appropriate growth media in it. For handling large numbers of transformed colonies, automated devices have been developed that locate the colonies on a plate and use robotic techniques to pick and inoculate cultures. When growing larger quantities of clones, it is common to inoculate isolated colonies into standard 96 well microtiter plates or alternatively 96 well culture blocks which can hold more than 1 mL of liquid culture medium. In existing methods, the container used for cell culture is used exclusively for that purpose and subsequent sample processing necessarily requires transfer of the cellular material to an alternative container.
The growth media in the wells of the plate is used to grow more of the particular bacteria with the particular plasmid of interest. Typical growth media include: 2xYT, TB (Terrific Broth), and LB (Luria-Bertani); others will occur to those of skill in the art. Typically, the bacteria are allowed to grow for about 12 to about 24 hours.
After the growth in the plate, the bacteria are harvested. That involves, typically, centrifugation (e.g., for 5 minutes). Centrifugation causes the bacteria, which are heavier than the growth media, to sediment to the bottom of the centrifuge tube. The growth media, which is generally liquid, is then poured or pipetted out of the wells of the plate.
A liquid (so-called “buffer”) is then added to the wells, and the wells are agitated to re-suspend the cells. A common method used to purify plasmid DNA molecules is the alkaline lysis method. In this procedure cells are initially resuspended in a Tris-HCl buffered saline solution. They are then lysed, or ruptured by adding an alkaline (typically NaOH) solution to cause the bacteria to break open, in order to free the plasmid from the bacteria. Then a third solution, a neutralization solution, for example a sodium or potassium acetate solution, is added to the lysed cells to neutralize the alkali.
This is a key step that also causes precipitation of unwanted cell components, in particular chromosomal DNA and proteins. A centrifugation step then occurs to further separate the unwanted material. The supernatant that results from the centrifuge includes desired plasmids. The precipitate does not. So the supernatant is drawn off by pipetting or some other means. Plasmid DNA can be further purified and concentrated from this neutralized solution, for example by phenol chloroform extraction and ethanol precipitation, or alternatively by adsorption of the plasmid DNA to a DNA binding substrate such as a silica resin. Plasmid adhered to silica resin is generally processed by sequential washing, drying and elution steps.
In addition to the problems previously discussed regarding the need for a single-container method and apparatus, generally, the preparation of polynucleotides (e.g. plasmids) has suffered from inefficiently-designed process steps, unsophisticated combinations of substances, and the use of various devices that have not lent themselves to efficient processing. This is particularly an issue when it is necessary to prepare larger and larger numbers of plasmid templates for high throughput genomic analysis. There is a long-felt need, therefore, for an apparatus that allows for multi-step processing in a reduced number of reaction chambers, automated handling of the reaction chambers, and for processes and systems that run in a more simplified and automated manner.
Various example embodiments of the invention address at least one of the needs described above, as well as other needs that those of skill in the art will recognize, although each example of the invention does not necessarily address all of the needs described above. Each of the examples has its own object(s); they will be apparent to those of skill in the art.
In at least one example of the invention, a device is provided for processing containers having a plurality of biological sample wells wherein at least one of the wells includes a biological sample. The device comprises processing stations, a sample guide between the at least two processing stations, and an actuator of the container from at least one processing station to at least another processing station. Various examples of processing stations include but are not limited to, a processing “plate” dispenser (as sometimes used in the art, “plate” generally refers to containers having multiple sample vessels or wells), a processing plate agitator, and a processing fluid dispenser. In at least one example, the processing fluid dispenser comprises a set of injectors. In at least one more specific example, the injectors are recessed. In a further example, they are stationary. In still a further example, the processing fluid dispenser comprises: at least one reservoir comprising; a biological substance process input port and a plurality of dispense ports; and a set of dispensing protrusions connected to the dispense ports. In some examples, the plurality of dispense ports is arranged in a substantially two-dimensional array. In some further examples, the reservoir comprises a cross-section that tapers from the input port, which allows air in the supply or from the dispense needles to gather above the fluid to be dispensed (which is vented through a valve or other means for removal of air or reduction of pressure in some further examples).
In at least one example of the invention, dispensing protrusions are recessed in a guard member (for example, a set of elongated recesses from the dispensing protrusions).
In still a further example of the invention, at least one of the processing stations comprises a processing plate piercer, and in still a further example, at least one of the processing stations comprises a pressure aperture and a seal positioned and arranged for interaction with the container.
In still another example, at least one of the processing stations comprises a collector plate dispenser and/or a collector plate sealer.
In even further embodiments, the at least two processing stations comprise at least two multi-sample, biological sample container processing stations, guides between the at least two multi-sample, biological sample container processing stations, and/or stops at a plurality of the at least two multi-sample, biological sample container processing stations.
In some such examples, a slideable actuator is mounted between the at least two processing stations.
In still another aspect of the invention, a system is provided for treatment of a plurality of biological samples in a multi-sample container, the system comprising: means for moving a first multi-sample container to a first processing station; means for processing the first multi-sample container at the first processing station; means for moving the first multi-sample container to a second processing station; means for moving a second multi-sample container to the first processing station; means for processing the first multi-sample container at the second processing station; and means for processing the second multi-sample container at the first processing station.
In at least one such system, the means for moving the first multi-sample container is operated during at least a portion of the moving the second multi-sample container. In a further example, the means for processing the first multi-sample container at the second processing station occurs during at least a portion of the processing of the second multi-sample container at the second processing station. In still a further example, the means for processing the first multi-sample container at the first processing station comprises means for contacting a processing fluid with the biological samples in the first multi-sample container (e.g., means for injecting the processing fluid into the first multi-sample container and/or means for maintaining a substantially laminar stream). In at least one specific example, the means for injecting comprises means for isolating injectors from the sample container (e.g., the means for isolating comprises means for recessing injectors in a dispensing head and/or means for controlling relative amounts of processing fluid dispensed into each of the biological samples). In at least one more specific example, the means for controlling comprises means for supplying processing fluid to multiple injection conduits from a proximate reservoir and a supply conduit. In some even more specific examples, the means for supplying processing fluid to the proximate reservoir comprises a pinch actuator on a supply conduit and/or a peristaltic actuator on a supply conduit.
In still another example of the invention, the means for processing the first multi-sample container at the first processing station comprises means for agitating the first multi-sample container (e.g., a “vortexer” as is commonly known).
In at least one example, the first processing station comprises means for creating an aperture for at least one sample in the first multi-sample container, or for example, for each sample in the multi-sample container (e.g., a piercer, using an elongate member.
In still a further example, the means for processing comprises means for removing of a fluid through the aperture (e.g., drawing or pushing air from the aperture with a positive or negative pressure pump).
In some examples of the invention, the means for moving comprises means for pushing the multi-sample container (e.g., a linearly-actuated member comprising a multi-sample container contact member, wherein the contact member is positioned and arranged for pushing the multi-sample container).
In at least one example, the means for moving comprises means for sliding (e.g., a track having means for guiding the multi-sample container from the first processing station to the second processing station and/or stops for positioning the multi-sample container at the first processing station and at the second processing station.
In some examples, at least one processing location comprises a means for sealing the multi-sample container at a given processing location.
In another example, a system is provided as noted above wherein at least one of the processing locations comprises a pressure change aperture and at least one of the processing locations comprises an agitator or shaker (e.g., the vortexer mentioned before). Some further examples include a collection container dispenser. positioned and arranged to place a collection container under the processing plate. In some such examples, the collection container dispenser further comprises a pressure change aperture with a seal for the collection container.
Still further examples of the invention include at least one processing station comprising a processing plate dispenser.
In still another aspect of the invention, a method is provided for treatment of a plurality of biological samples in multi-sample container, the method comprising: moving a first multi-sample container to a first processing station; processing the first multi-sample container at the first processing station; moving the first multi-sample container to a second processing station; moving a second multi-sample container to the first processing station; processing the first multi-sample container at the second processing station; and processing the second multi-sample container at the first processing station.
In at least one example, the moving the first container occurs during at least a portion of the moving of the second container. In a further example, the moving the first multi-sample container occurs during at least a portion of said moving the second multi-sample container. In yet another example, the processing the first multi-sample container at the second processing stations occurs during at least a portion of said processing of the second multi-sample container at the second processing station. In even further examples, the processing the first multi-sample container at the first processing station comprises contacting a processing fluid with the biological samples in the first multi-sample container (e.g., injecting the processing fluid into the first multi-sample container while maintaining a substantially laminar stream and/or isolating injectors from the sample container). In at least one example, the isolating comprises recessing injectors in a dispensing head. In still a further example, the means for isolating comprises means for controlling relative amounts of processing fluid dispensed into each of the biological samples (e.g., supplying processing fluid to multiple injection conduits from a proximate reservoir through a supply conduit).
In yet a further example, the processing the first multi-sample container at the first processing station comprises agitating the first multi-sample container and/or creating an aperture for at least one sample in the first multi-sample container. In some such examples, the creating comprises piercing a re-sealing or non-resealing material. In further examples, the processing also comprises removing of a fluid through the aperture (e.g., creating a pressure differential between an interior well of the multi-sample container and the aperture, wherein the pressure is greater in the well than at the aperture by drawing or pushing air)
In still further examples, the moving comprises urging along a track by pushing, pulling, and/or sliding.
In an even further example of the invention, a system is provided for harvesting polynucleotides from a growth plate in which bacteria that include the polynucleotides reside and in which growth media reside. The system comprises: means for inserting into the growth plate a lysis fluid; means for agitating the lysis fluid and bacteria in the growth plate; means for creating an aperture in the growth plate; means for inserting a wash fluid into the growth plate; means for passing a gas through the growth plate; means for inserting a solubilizing fluid into the growth plate; and means for creating a pressure differential across the processing plate whereby DNA is removed from the growth plate.
In some examples, the lysis fluid comprises a buffer. In further examples, the lysis fluid comprises a substantially neutral pH. In still further examples, the lysis fluid comprises a non-alkaline fluid. In yet further examples, the lysis fluid comprises a salt (e.g., an acetate-containing salt consisting essentially of a TRIS acetate salt). In some examples, the salt consists essentially of a chaotropic salt.
In still further examples, the lysis fluid comprises a detergent.
In even further examples, the wash fluid comprises a buffer and/or an enzyme (e.g., an RNA-specific enzyme and/or a non-DNA specific enzyme). In some examples, the wash fluid poorly solubilises DNA. In still further examples, the wash fluid solubilises lipids, chaotropic salts, and carbohydrates, faster than the wash fluid solubilises DNA. In still further examples, a majority of the wash fluid comprises alcohol (e.g., between 30% and 98% by volume). In yet a further example, the solubilizing fluid comprises water.
In yet further examples, the gas comprises air.
In an even further example of the invention, there is provided a means for removing the wash fluid from the growth plate and a means for reinserting the wash fluid into the growth plate. In at least one example, the means for removing and means for reinserting operate before said means for passing a gas. In at least one other example, the means for removing and the means for reinserting occur after said passing a gas.
In still a further example, the system further comprises means for holding the wash fluid in the growth plate for a period long enough for an enzyme in the wash fluid to degrade RNA from silica in the growth plate (e.g., between about one minute and about five minutes).
Foam can also be a problem in some examples, and to avoid that formation, in some examples of the invention, a means is provided for preventing foam that comprises means for removing air from contact with the lysis fluid in the growth plate during removal of the lysis fluid. In at least one example, the means for removing air comprises means for inserting of the wash fluid into the growth plate before the removal of the lysis fluid.
In yet a further example, the means for inserting the wash fluid operates before said means for removing the lysis fluid.
In still a further example, a means is provided for inserting a further wash fluid after removal of the wash fluid having an alcohol content greater than the alcohol content of the wash fluid. In at least one example, the means for passing a gas comprises means for pulling air through the growth plate. In another example, the means for passing a gas comprises means for pushing air through the growth plate.
In yet another example, the means for inserting a solubilizing fluid in the growth plate comprises means for inserting water in the growth plate and/or the means for creating a pressure differential comprises means for placing a collection plate near the aperture and drawing a gas from at least one edge of the collection plate.
In still a further example of the invention, a method is provided for harvesting polynucleotides from a growth plate in which bacteria that include the polynucleotides reside and in which growth media reside, the method comprising: inserting into the growth plate a lysis fluid; agitating the lysis fluid and bacteria in the growth plate; creating an aperture in the growth plate; inserting a wash fluid into the growth plate; passing a gas through the growth plate; inserting a solubilizing fluid into the growth plate; and creating a pressure differential across the processing plate whereby DNA is removed from the growth plate.
In at least one example, the method further comprises removing the wash fluid from the growth plate and reinserting the wash fluid into the growth plate. In some such examples, the removing and reinserting occur before said passing a gas. In some other examples, the removing and reinserting occur after said passing a gas.
In still other examples, the method further comprises, holding the wash fluid in the growth plate (e.g., for a period long enough for an enzyme in the wash fluid to degrade RNA from silica in the growth plate).
In still another example, the method further comprises preventing foaming of the lysis fluid during removal of the lysis fluid (e.g., by removing air from contact with the lysis fluid in the growth plate during removal of the lysis fluid). In at least one such example, the removing of air comprises insertion of the wash fluid into the growth plate before the removal of the lysis fluid (e.g., before removing the lysis fluid). In some such examples, the method further comprises inserting a further wash fluid after removal of the wash fluid.
In some further examples, the passing a gas comprises pulling and/or pushing air through the growth plate.
In still further examples, the inserting a solubilizing fluid in the growth plate comprises inserting water in the growth plate and the creating a pressure differential comprises placing a collection plate near the aperture and drawing a gas from at least one edge of the collection plate.
According to yet another example of the invention, a biological sample preparation device (sometimes known as a “plate”) is provided comprising: a plurality of reaction volumes wherein each reaction volume is in a fixed relation to other reaction volumes; and a recessed sample extraction location for each reaction volume. Each of the recessed sample extraction locations comprises at least one projection beyond each of said recessed sample extraction locations.
In at least one example of the invention, a skirt resides around the recessed sample extraction locations and comprises a sealing edge. In at least some examples of the invention, an elongate member resides around each of said recessed sample extraction locations and as any of a variety of cross-sectional shapes (e.g., cylindrical, or other curved shape and/or polygonal shape, such as a triangle, parallelogram, rectangle, square, pentagon, hexagon, etc.).
In some examples, the reaction volumes comprise an open end of the reaction volume (which is an elongate shape).
In yet other examples, the reactions volumes are spaced from each other with spacer members between said plurality of the reaction volumes, while, in still further examples, the reaction volumes reside in a substantially unitary structure defining said plurality of reaction volumes and defining said recessed sample extraction location for each reaction volume. An openable, centrifugal sample extraction member located at each of said recessed sample extraction locations that comprises a piercable material is provided in some examples (e.g., a plastic). In some examples, the openable member is of a soluble and/or meltable material. In still further examples, the material is photo-reactive material.
In still a further example of the invention, a binding material (e.g., silica) is present in the reaction volumes. For example, in some embodiments of the invention, lysing and binding of polynucleotides occurs in one location in substantially the same process step. Diatomaceous earth is used in at least one example, and a powder form of a binding material is used in further examples. In some examples, the binding material comprises silicon dioxide. In further examples, polynucleotide growth media resides in at least one of the plurality of reaction volumes, and silica and polynucleotide growth media reside in at least one of the plurality of reaction volumes in still further examples.
In a further example of the invention, a system is provided for producing a plurality of polynucleotides from at least one colony of host cells, the system comprising: means for maintaining a reaction volume for each polynucleotide; means for maintaining a distance between the reaction volumes; means for receiving the plurality of polynucleotides in the reaction volumes; and means for providing a sample extraction path from each reaction volume.
In at least one such system, the system further comprises means for providing at least one recess of at least one sample extraction path (e.g., at least one projection beyond said means for providing at least one sample extraction path). In some examples, the at least one projection resides between a plurality of means for providing a sample extraction path, around a plurality of means for providing a sample extraction path, or around all of the means for providing a sample extraction path.
In some examples, the at least one projection comprises a single projection around all of the means for providing a sample extraction path or multiple projections wherein said multiple projections, together, define a recess in which there resides plurality of means for providing a sample extraction path. In at least one example, the means for providing at least one recess of at least one sample extraction path comprises a skirt around all the means for providing a sample extraction path from each reaction volume.
In yet another example of the invention, a device is provided comprising: at least two multi-sample, biological sample container processing stations; guides between the at least two multi-sample, biological sample container processing stations; and stops at a plurality of the at least two multi-sample, biological sample container processing stations.
In some examples, at least one processing station comprises a seal positioned and arranged for contact with a sample container. In further examples, the least one processing station comprising a seal further comprises a pressure aperture. In still further examples, a slideable actuator is provided that is mounted between the at least two processing stations.
In still another example of the invention, a system is provided for manipulation of multi-sample biological sample containers, the system comprising: means for receiving a first sample container, at a first processing location; means for guiding the first sample container to a second processing location; means for holding the first sample container at the second processing location; and means for receiving a second sample container at the first processing location.
In at least one example, the system further comprises means for pushing the multi-sample container between the first and the second processing locations (e.g., a linear motion actuator) such as an elongate member residing between the first and the second processing stations wherein the elongate member includes a protrusion slideably connected between the first and the second processing stations.
In at least one example, the system comprises means for pulling and/or means for pushing the multi-sample container between the first and the second processing locations and a means for sliding the multi-sample container between the first and the second processing locations.
In some examples, the means for sliding comprises a grooved track, and the means for receiving comprises a first recess in a track. In some examples, the means for guiding comprises guides along a track and the means for holding comprise stops in the track. In yet further examples, the means for receiving a second sample container at the first processing location comprise a second recess in the track.
In still another example of the invention, a method is provided, wherein the method is for manipulation of multi-sample biological sample containers. The method comprises: receiving a first sample container, at a first processing location; guiding the first sample container to a second processing location; holding the first sample container at the second processing location; and receiving a second sample container at the first processing location.
In at least one example, the method further comprises pulling and/or pushing the multi-sample container between the first and the second processing locations. In a further example, the method further comprises sliding the multi-sample container between the first and the second processing locations.
In still another example of the invention, a dispenser of biological substance process fluid is provided. The dispenser comprises a reservoir comprising: a biological substance process input port; a plurality of dispense ports; and a set of dispensing protrusions connected to the dispense ports.
In at least one example, the plurality of dispense ports is arranged in a substantially two-dimensional array, and the reservoir comprises a cross-section that tapers from said input port. In further examples, the dispensing protrusions are recessed in a guard member in a set of elongated recesses.
In a further example of the invention, a system is provided for dispensing a biological substance process fluid from a dispensing container to multiple samples of biological substances. The system comprises: means for receiving from the dispensing container a multiple sample amount of biological substance process fluid, wherein the multiple sample amount is sufficient for processing the multiple samples of biological substances; means for dividing the amount into a set of individual sample amounts in a multidimensional array; and means for substantially simultaneously dispensing the set of individual sample amounts to a set of individual samples.
In at least one example, the means for receiving comprises an accumulator of the multiple sample amount proximate a set of individual sample dispense paths. In a further example, the means for dividing comprises a manifold of individual sample dispense paths from a reservoir. In yet a further example, the means for dispensing comprises means for streaming the set of individual sample amounts to the multiple samples (e.g., an injector outside a container holding the multiple samples). In at least one more specific example, the means for streaming comprises a recessed injector that is substantially stationary during the receiving, dividing, and dispensing.
In still a further example of the invention, a method is provided for dispensing a biological substance process fluid from a dispensing container to multiple samples of biological substances, the method comprising: receiving from the dispensing container a multiple sample amount of biological substance process fluid, wherein the multiple sample amount is sufficient for processing the multiple samples of biological substances; dividing the amount into a set of individual sample amounts in a multidimensional array; and substantially simultaneously dispensing the set of individual sample amounts to a set of individual samples.
In at least one example, the receiving comprises accumulating the multiple sample amount proximate a set of individual sample dispense paths and the dividing comprises providing a set of individual sample dispense paths from a reservoir.
In still a further example of the invention, the dispensing comprises streaming the set of individual sample amounts to the multiple samples (e.g., injecting from outside a container holding the multiple samples).
In still a further example of the invention, a linear automated processing device is provided having at least two stations and performing a method for mixing (contacting two or more substances) in a plate the method comprising: introducing a plate; guiding the plate from a first station into a second station; said second station having a moveable portion; temporarily retaining the plate on said moveable portion; and imparting motion to said movable portion.
In another example of the invention, a method and system are provided for creating two or more apertures in a plate having two or more vessels each vessel comprising a nozzle portion, the method comprising: providing a plate; providing at least two means for creating an aperture; aligning at least two of the nozzle portions with a corresponding aperture creating means; guiding said at least two nozzle portions to contact a corresponding aperture creating means; and creating an aperture in at least two of the nozzle portions.
In still further examples of the invention, a reservoir area is provided to distribute the fluid being dispensed by the dispense nozzles and reduce the pressure gradient between nozzles due to the fluid flow. A plenum is provided and is constructed so as to provide a generally equal pressure at the inlet of all dispense nozzles and thereby improve accuracy. When air is trapped in the plenum area the compressibility of the air can cause dripping and inaccurate volumes to be dispensed. To aid in the removal of trapped air in the plenum, the dispense head reservoir comprises a sloped top area to allow trapped air to flow into and collect near the purge valve.
In yet another example, in a linear automated processing device having at least two stations a method is provided for uniting a first plate and a second plate, the method comprising: introducing a first plate into a first station; guiding the first plate from a first station into a second station; introducing a second plate into a second station; moving the first plate into the second station; moving the second plate underneath the first plate in the second station; and lifting the second plate to unite the second plate and the first plate.
In still another example, a linear automated processing device having at least two stations is provided using a method for transferring a substance from a first plate to a second plate, the method comprising: providing an assembly comprising a first plate and a second plate into a first station, said first plate comprising a substance to be transferred to the second plate; introducing said assembly into a first station; guiding the first plate from a first station into a second station; creating a differential pressure between the; moving the first plate into the second station; moving the second plate underneath the first plate in the second station; and lifting the second plate to unite the second plate and the first plate.
In yet a further example, in a linear automated biological sample processing device having a track and at least two stations a method is provided for transferring a plate from a first station to a second station, the method comprising: providing a track having a first station and a second station; introducing a plate into a first station; and transferring the plate from a first station into a second station while maintaining contact between the track and the plate.
In still a further example of the invention, a kit is provided for separating at least one target substance from a sample comprising biological cells, the kit comprising: one or more buffers comprising at least one re-suspension substance, at least one lysing substance, and at least one binding promoting substance; a retaining substance; and a container for receiving the cells, retaining substance and buffers such that when said cells, and buffers are contacted in said container re-suspension, lysis and binding to said retaining substance occur generally simultaneously.
An example embodiment of the current invention provides a kit for separating at least one target substance from a sample comprising biological cells, the kit comprising one or more buffers such as a re-suspension substance such as TE. Other suitable buffers as would be obvious to those skilled in the art can be substituted or the re-suspension substance could be eliminated and the lysing substance or binding promoting substance can be used as the re The kit also comprises a lysing substance.
In still a further example, there is provided a method for culturing cells and separating a target substance from the cells in the same container, the method comprising: providing a container for culturing the cells; providing cells to be cultured; culturing the cells in said container; introducing a retaining substance into the container; introducing a substance that aids retention of the target substance to the retaining substance into the container; introducing a substance that aids even dispersion of the cells and target substance into the container; introducing a substance that lyses the cells into the container; and contacting the cells and introduced substances in said container.
In even another example, a method is provided for separating a target substance from a substance comprising biological cells in a container, the method comprising: introducing the cells into the container; introducing a retaining substance into the container; introducing a re-suspending substance into the container; introducing a lysing substance into the container; introducing a binding promoting substance into the container; causing the cells to contact the re-suspending substance, lysing substance and binding promoting substance generally simultaneously.
In another example, a method is provided for improving the yield of a target substance from biological cells, the method comprising: providing a container; introducing into the container a mixture comprising a powdered substance, a growth media, and biological cells; and culturing the cells in said mixture.
In still a further example, a method is provided for separating a target substance from a substance comprising biological cells, the method comprising: providing biological cells; providing a retaining substance; lysing the cells; providing a retention promoting substance; contacting the cells and the lysing substance; and retaining the target substance in the presence of the products of said lysing.
In a further example, a method is provided for separating a target substance from a substance comprising biological cells, the method comprising: introducing a lysing substance into the container; introducing a retaining substance into the container; contacting the cells and the lysing substance; providing a retention promoting substance; and retaining the target substance in the presence of the products of said lysing.
A method is also provided for improving the separation of a target substance from a mixture comprising biological cells and a supernatant in a container, the method comprising: providing a container; introducing a substance comprising biological cells into the container; introducing a powdered substance into the container; and separating cells and powder from the supernatant.
Still another method that is provided according to another example of the invention is a method for removing impurities while separating a target substance from a substance comprising biological cells, the method comprising: providing a container having at least a sample introducing end and a supernatant removal end; introducing a retaining substance into the container; introducing a biological cells lysate into the container; contacting the cell lysate and the retaining substance in the container; introducing a wash buffer so as to separate the cell lysate from the sample introducing end; creating a differential pressure between the sample introducing end and the supernatant removal end; and passing the cell lysate past at least a part of the retaining substance and through the supernatant removal end while maintaining separation of the cell lysate from the sample introducing end with the wash buffer.
A wash buffer is provided in still another example for removing unwanted substances from a sample comprising at least one target substance and at least one unwanted substance, the buffer comprising an enzyme for digestion of the unwanted substances.
A further method that is provided is a method for washing a mixture comprising a target substance and at least one un-wanted substance, the method comprising: contacting the mixture with a wash buffer comprising an enzyme capable of degrading said at least one un-wanted substance; allowing the enzyme to degrade said un-wanted substance; and removing said wash buffer from said mixture.
In at least one example of the invention, a plate is provided that can bind the target substance (such as DNA, RNA, proteins, etc.) and that is compatible with cells to be grown. In at least one example, a plate includes a sealed bottom (nozzle) that can bind the target substance. (such as DNA, RNA, proteins, etc.).
Further example embodiments will occur to those of skill in the art, and the above are given by way of example only.
Referring now to
Referring now to
During operation, in at least one example of the invention, actuator 15, shown in
During operation of the device of
Referring now to
Referring now to
Wells 531-539 are a small subset of the 96 wells. It should also be noted that although many wells are shown as circular cylinders, in various example embodiments, the shape of each, several, or all wells may be varied as is shown by wells 531-539. In at least one example embodiment of the present invention, wells 531-539 comprise a hollow cylindrical body having an open end and a spherical closed end. In another example embodiment, all processing wells are made of a thermoplastic material. In other embodiments, any suitable material and any suitable shape that will occur to those of ordinary skill in the art is used. Referring now to
It should be noted that although 96 wells are shown, the number of wells can be greater than or less than 96 and may be arrayed differently than illustrated in
Referring to
In various examples, the processing stations 2 are in various forms. For example, in the example illustrated in
Referring now to
In some examples of the present invention, escapement mechanism 120 is held into an initial “closed” position, as shown in
In some examples of the present invention, a stripping piston 150 is used to dislodge processing container 3 from containers above 3, not shown, that processing container 3 has become “stuck” to. Stripping piston 150, as illustrated in
Referring now to
It will be noted that in the illustration, the guard member comprises a set of elongated recesses from said dispensing protrusions. In at least one alternative example of the invention, the guard member 220 comprises a set of polygonal shapes (e.g., triangles, rectangles, squares, hexagons, etc.). In some such examples some dispensing protrusions reside in the same recess. In other examples, each dispensing protrusion resides in an individual recess, while, in still further examples, all dispensing protrusions are guarded in a single recess. Multiple variations and combinations are available in still further examples that will occur to those of skill in the art.
Referring now to
In at least some examples of the invention, when a processing plate, not shown, is located on the shaker plate 300, the processing plate is aligned with the dispensing protrusions, not shown, from fluid dispenser 340 so that fluid is delivered to the processing plate wells without spillage. In some example embodiments of the invention, this alignment is achieved via a shaker plate alignment device 360. Referring now to
In some examples of the current invention, a processing plate is secured to the shaker plate to prevent the processing plate from being shaken off the shaker plate during agitation. In one such example, gripper 440, identified as 370 in
In some example embodiments, gripper 440 is pulled away from the base of a given processing plate, not shown, when alignment cone 410 is lowered into rough alignment cone 420.
During operation, in one example embodiment, prior to delivery of a processing plate to shaker plate 400, alignment cone 410 is seated at the base of alignment shaft 430, aligning shaker plate 400 with fluid dispenser 405 and retracting gripper 440. A processing plate, not shown, is then delivered to shaker plate 400. To begin agitation, alignment cone 410 is raised, releasing shaker plate 400, allowing gripper 440 to grip the processing plate to hold it on shaker plate 400, and eccentric bolt 416 is rotated.
Referring now to
Referring now to
Referring now to
Referring now to
Referring now to
During operation, in at least one example,
In at least some examples of the invention, dispensing micro titer plates is performed with the same mechanism illustrated by
Referring now to
Referring now to
In some embodiments of the present invention, microtiter plates consist of 96 collection wells arrayed and held in relation to each other by plate 473. In some example embodiments, collection wells comprise a cylindrical body having an open end and a spherical closed end. In other embodiments, plate 473 and collection wells are made from a single part. In another example embodiment, the collection wells and plate 473 are made of a thermoplastic material. In other embodiments, any suitable material and any suitable collection well shape that will occur to those of ordinary skill in the art is used. To allow efficient collection during operation in some example embodiments, the collection plate well array is matched to the well array in a given processing plate such that when a given microtiter plate is aligned below a given processing plate, processing plate wells and collection plate wells align such that any fluid or other materials exiting processing well apertures is collected by the collection wells.
During operation, as illustrated in
In at least one alternative embodiment of the present invention, illustrated in
Referring now to
Looking again at
Referring now to
In a further description of the examples seen in
Referring again to
In a further example, the means for moving comprises a rotating wheel 998 with at least one push rod 1002, as illustrated by
In yet another example, the means for moving comprises a conveyor belt, as illustrated by
In at least one example, the means for moving the first multi-sample container is operated during at least a portion of the moving of the second multi-sample container; in a further example, the means for processing the first multi-sample container at the second processing station occurs during at least a portion of the processing of the second multi-sample container at the first processing station.
In a further example of the system illustrated in
Such an arrangement provides for accurate placement of the processing fluid in the well in which the biological sample resides without the need to insert the injector in the well. This is in contrast to some previous methods of dispensing biological sample fluids into processing wells, in which pipettes or other systems were used with disposable tips. Due to concern that the tips are contaminated during insertion into the well, the tips are discarded after each dispensing step, leading to a disposal problem of potentially hazardous biological waste. Other shapes and stream characteristics will occur to those of skill in the art.
In at least one example of the invention, as seen in
Referring now to
Referring now to
Referring now to
In at least one, more specific example of the invention, seen in
In still a further example of the invention, seen in
In still a further example of the invention, the means for moving comprises means for pushing the multi-sample container. In at least one such example, the means for moving comprises a linearly-actuated member comprising a multi-sample container contact member positioned and arranged for pushing the multi-sample container; in another example, the contact member is positioned and arranged for pulling the multi-sample container. In some examples, a slideable surface or means for sliding is a component of the means for moving; in some such examples, the means for sliding comprises a track having means for guiding (e.g., sample guides 521 and 523 in
Referring now to
In still a further example of the invention, seen in
In at least one example, collection container 453 mates with processing container 451 in a manner that allows air to flow around collection container members (
Referring now to
In still a further example, the at least one projection resides around at least one of each of said recessed sample extraction locations; and, in still another example, the projection resides around only one of said recessed sample extraction locations.
In still a further example, there are multiple projections wherein each of the multiple projections resides around at least one of said recessed sample extraction locations. In another example, each of the multiple projections resides around only one of each of said recessed sample extraction locations.
In
The cross-sectional shape of the elongate members forming recesses varies in a number of examples. A non-exclusive list of acceptable shapes comprises: curved (including cylindrical) and polygonal (including triangles, rectangles, squares, pentagons, hexagons, etc.) some of which are shown in
As seen in the illustrated example in
In many example embodiments, the reaction volume comprises an openable, centrifugal member in which a substance is centrifuged in some examples, and opened by various means in further examples. As mentioned before, in at least one such example, the reaction volume is openable to provide a sample extraction location by piercing. In some such examples, there is a piercable material (e.g., plastic), and in some more specific examples, piercable material is re-sealing, while, in others, it is not re-sealing. Some further examples include the use of a break-away member (e.g., a hinged flap), a soluble material, a meltable material, a cap, and/or a photo-reactive material.
In many embodiments, at least one of the plurality of reaction volumes includes retaining material such as silica. As mentioned elsewhere, the growth of biological materials in the presence of retaining material has a benefit of removing a processing step from some methods of processing biological materials. There are further benefits, also. In some instances, the retaining material comprises diatomaceous earth; in further examples, the retaining material comprises silicon dioxide; in further examples, the retaining material comprises glass beads; in further examples, the retaining material is a material that comprises chromatographic media; in still further examples, the retaining material comprises a glass filter. Other forms of silica or binding material useful in various examples of the invention will occur to those of skill in the art.
In some further examples, growth media resides in at least one of the plurality of reaction volumes. Various growth media are useful, depending on a variety of factors. A non-exclusive list of useful growth media includes 2xYT, TB (Terrific Broth), LB (Luria-Bertani) and others for the culture of eukaryotic and/or prokaryotic cells such as bacterial, mammalian, plant and other cell types as will occur to those of skill in the art.
A further explanation of the example of
In some examples (e.g.
As shown in
In still another example (e.g.,
In another explanation of various examples, in
In the illustrated example in
Also in the illustrated example, the means for maintaining a reaction volume for each sample comprises an elongate member 465. In some such examples, the reaction volume includes a cross-sectional area having a curved shape, while, in further examples, the elongate reaction volume has a polygonal cross-section.
In a further example, the means for receiving the plurality of samples in the reaction volumes comprises an open end 475 of the reaction volume.
In an alternative description of the example of
In a further description of an example of the invention as seen in
Some examples of the invention also include means for pushing the multi-sample container between the first and the second processing locations (e.g. an actuator), in the illustrated example in
The actuator of
In the present description, in some embodiments of the present invention, the means for guiding comprises guides along a track, the means for holding comprise stops in the track, and the means for receiving a second sample container at the first processing location comprise a second recess in the track.
In another description of a further aspect of the invention, a system is provided for dispensing a biological substance process fluid from a dispensing container to multiple samples of biological substances. As seen in
In the example of
In at least one example embodiment of the invention, a system and method for harvesting polynucleotides is provided. In one such system and method the combination of an alkaline lysing buffer and gentle agitation to re-suspend are not used. Rather, in this example of the invention, a non-alkaline buffer is used (substantially neutral pH—e.g., in one example embodiment, 5M Guanidine Solution 1% Sarkosyl is composed of the following reagents in the following proportions for every liter of fluid: 590 gm Guanidine isothiocyanate; 25 ml 1M Tris-HCL, pH 8.0; 10 ml 0.5 M EDTA; 50 ml 20% Sarkosyl; to up to 1000 ml ddH2O; eliminating the need for a neutralization buffer). It has been found that a problem with an alkaline buffer is that it will destroy the DNA if left in too long. It has also been found that using 5M Guanidine Solution 1% Sarkosyl, in certain embodiments of the present invention, allows for resuspending, lysing, and binding in a single step.
After insertion of the non-alkaline lysis buffer into the wells, in the present example of the invention, the wells are agitated/vibrated (sometimes referred to as “vortexed” because in a cylindrical well, a vortex will result) to mix the lysis buffer with the bacteria to increase the speed of reaction with the multiple bacteria and the number of bacteria that are actually lysed. In at least one example of the invention, the agitation is vigorous (e.g., refer to
After the cells have been lysed, there is a mixture in which the plasmids and other cell parts are suspended. In the presence of the lysis buffer, the DNA binds to a silicate surface. In some processes, a solution resulting after lysis (including lysis buffer and open cells) is transferred to another chamber having silicate; however it is an improvement provided by at least one example of the invention to grow the bacteria in the presence of silicate. In at least some examples, the bottom of the wells of the plate are pierced and the lysis buffer fluid is pulled out, leaving the DNA bound to the silicate left in the plate. In many instances, the silicate is put in the wells before the growth media and bacteria are inserted. In other example embodiments of the invention a material other than silicate may be substituted for binding the DNA as will occur to those of skill in the art. Some example alternative binding materials include ion exchange resins, silicon carbide and other media suitable for liquid chromatography applications.
Also, in some systems in which there is a transfer of the solution having lysis buffer and open cells from the wells to another chamber, the other chamber includes chaotropic salt and silicate. In at least one example of the invention, chaotropic salt is inserted in the wells with the lysis buffer. Or, said another way, in some examples of the invention, the lysis buffer includes a chaotropic salt, non-chaotropic salt or other binding promoting substance as would occur to one skilled in the art, to help the polynucleotide of interest (e.g., DNA) to bind to the silicate or other binding media. Some example binding promoting substances or agents are: guanidinium thiocyanate; guanidinium hydrochloride; sodium chloride; potassium chloride; sodium perchlorate; potassium iodide; and sodium iodide. Growing the bacteria in the presence of silicate and adding the salt to the well in which the growth and lysing occurs avoids the need to transfer the resulting post-lying solution to another chamber. In at least one example of the invention, a chaotropic salt or other suitable salt or other suitable binding promoting agent, as would be apparent to one skilled in the art, is inserted in the wells with the lysis buffer and the resulting mixture is then transferred to another vessel and contacted with a binding media such as silicate or other suitable material which binds DNA.
In that post-lysing solution, there is still a lot of material, that is not of interest, still left in the wells, even after the piercing and removal of the lysis buffer. To separate the polynucleotides of interest from the other material, a “wash buffer” is added to the well, which will carry away the cell wall and other parts that are not wanted. In at least one example, the wash buffer comprises a solution in which DNA has low solubility, but other items that are not of interest have a high solubility. For example, high-alcohol-content solution will wash away lipids, chaotropic salts, carbohydrates, and other cell debris and non-desirable items, but DNA is poorly soluble in an alcohol solution. One example of a suitable wash buffer is a 50% wash solution with RnaseA composed of the following proportions per 2.5 liters of solution: 100 ml 1M Tris Acetate pH 7.0, 50 ml 2M Sodium Acetate, 5 ml RnaseA, to 2350 ml dH2O.
In at least one example of the invention, the lysis buffer includes a detergent that aids in solubilization of cell walls (e.g., sarkosyl, Tritron X-100, SDS, Pluronic L61 made by BASF, IGEPAL, and others that will occur to those of skill in the art). However, in some embodiments, when the well is evacuated, and the column of the lysis buffer reaches the bottom of the well, there is air and lysis buffer. A foam is generated that can build upward and contaminate the sample. Therefore, according to still another example of the invention, rather than pulling the lysis buffer out and then putting wash buffer in, the wash buffer is inserted in the well on top of the lysis solution (after agitation, before evacuation of the lysis buffer). In such a manner, air is isolated from the lysis solution in the well, and there is no foam. In addition to the contamination caused by the foam coming back up the lower evacuation area, the silicate contained residual lysis buffer that, in contact with air, would contaminate the DNA bound in the silicate. The wash buffer passing though the silicate, that is holding the DNA, removes the lysis buffer also from the silicate. Therefore, the first time after lysing that air contacts the silicate, there is no residual lysis buffer in contact with the silicate to cause a foam contamination.
In some further examples, the wash buffer also contains an enzyme that will degrade unwanted RNA (bound with the silicate just as the desired DNA). In some such examples, the wash buffer solution is passed through the well again, leaving it in for a period of time to allow it to work on the RNA.
According to still further examples of the invention, a further wash buffer solution that has a higher alcohol than the first wash buffer follows the first wash buffer solution (which, as discussed above, is used twice in some examples). One example of a suitable further wash buffer solution is an “80% wash solution” composed of the following proportions per 1.0 liter of solution: 100 ml 1M Tris Acetate pH 7.0, 50 ml 2M Sodium Acetate, to 850 ml dH2O. Air is then caused to flow through the resulting “cake” of silica having the DNA bound to it (to dry the alcohol out). That leaves dry silica with DNA bound to it.
In further embodiments, water is added, which rehydrates the DNA into solution from the silicate.
In still further examples of the invention, a collection plate (a so-called “microtiter” plate in some examples) is set under the processing plate that holds the wells. In some further examples, a centrifuge step drives the DNA solution to the collection plate; in other examples, a vacuum method is used in which an interlocking chimney, as seen in
In still a further example of the invention, the collection plate is sealed so that stacking can occur for storage.
In still a further example of the invention, in the collection plate, there is another precipitation step that occurs to further concentrate the DNA. However, it is believed that no such precipitation step is required with the broader examples of the invention; at least with most plasmids, the plasmid DNA is concentrated in the collection plate enough that the further precipitation step is unneeded. Part of the reason for this is the use, in some examples, of a TRIS acetate in the wash buffer. In some example embodiments, the wash buffer is made of between 5% and 25% by volume of TRIS acetate. In other example embodiments, the wash buffer is made of approximately 10% by volume of TRIS acetate. In other example embodiments and at differing wash steps within the process described above, the wash buffer or wash solution is made of between 0.5% and 10% by volume of TRIS acetate. In other example embodiments, the wash buffer is made of approximately 4% by volume of TRIS acetate. That substance conditions the silica for easier DNA release when water contacts the dried silica. A number of salts are considered useful, although chloride salts have been found not to work as well as acetate-containing salts. Acetate-containing salts are predicted to work better than chloride salts.
In another example embodiment of the invention, a system and method for harvesting M13 DNA is provided. M13 bacterial cultures are incubated in at least one processing plate 3 (illustrated in
After the incubation, in a further embodiment, the processing plate 3 is vortexed, as described above and illustrated by
Next, a second reagent is added to the wells, in the present embodiment this is done to dissociate the phage proteins from the DNA and a volume of approximately 5.2 milliliters is added. An example second reagent is any de-kaotropic salt solution such as a 6.5M sodium per-chlorate solution composed of the following reagents in the following proportions: 456.63 gm Sodium Perchlorate (Sigma Cat. #51401-500G); 5 mls of 1 M tris-HCL (pH 8.0); 100 micro-liters of 0.5 M EDTA (pH 8.0); QS to 500 mls with sterile H2O. Next, a vacuum is again applied to the closed end of the processing plate to remove the Sodium Perchlorate solution. The DNA is now bound to the filters in the wells. Next, a third reagent is added to the tube or vessel, to wash the excess proteins, salts and other debris from the filter-bound DNA. One example of a suitable third reagent is a 75% Ethanol solution composed of the following reagents in the following proportions: 525 ml of 100% Ethanol (200 proof AAPER Alcohol & Chemical Co., DSP-KY 417); 175 ml sterile H2O. Next, a vacuum is applied to remove the ethanol, in a manner similar to the previous steps.
Next, a fourth reagent is added to the wells. One example of a suitable fourth reagent is any substance that comprises a biological suspension buffer and a divalent cation scavenger such as TE buffer. A suitable quantity for the example TE buffer is 45 micro-liters and comprises the following reagents: Tris (hydroxymethyl) aminomethane (TRIS) and ethylenediaminetetraacetic acid (EDTA). Next a vacuum is applied to the closed end of the processing plate to elute the DNA into a sample container, not shown. The pressure differential across the aperture forces the eluted DNA from the filter through the aperture, and into the container, not shown. The purified DNA is ready for further amplification, sequencing, testing, or storage. The processing container is discarded.
Various steps of the example embodiments of the invention involve forcing fluid through the aperture in the processing plate wells under the influence of a pressure differential across the aperture. In various embodiments, vacuum, positive pressure, or any other method that will occur to those of ordinary skill in the art is used in any of these steps to create the necessary pressure differential. In other embodiments, any suitable means that will occur to those of ordinary skill in the art such as inertia or centrifugal force are used to force the fluid to exit the processing plate wells. In still a further embodiment, the elution of substances such as DNA, RNA or other desired substances as will occur to those of ordinary skill in the art is also accomplished by centrifugation.
Some embodiments of the invention relate to any application where a desired substance is sought to be isolated, extract, or otherwise processed from a sample substance, solid, plasma or gas, containing the desired substance and one or more waste substances. In various embodiments, a desired substance is a protein, DNA, RNA, or any other macromolecule or combination thereof that will occur to those of ordinary skill in the art. In some instances, it may not be necessary to pellet the precipitate.
In yet another example embodiment of the invention, a system and method for harvesting bacterial plasmid DNA is provided. In one example embodiment, bacterial cultures are incubated in a least one processing plate. Cells are harvested in the processing plate by centrifugation at 2500 g for 5 minutes. The supernatant is carefully poured off or pipetted out of the processing plate. In at least one other example embodiment cell harvesting by centrifugation or other means is omitted and lysis buffer is added directly to the culture media containing the target cells. In at least one embodiment, 200 uL of a first reagent is added to each well in the processing plate to resuspend and lyse cells. An example first reagent is composed of the following reagents in the following proportions: 295 g Guanidine isothiocyanate; 12.5 ml 1M Tris-HCL, pH 8.0; 5.0 ml 0.5 M EDTA; 25 ml 20% Sarkosyl; to 500 ml dH20. The processing plate it vortexed vigorously for one minute. Next, the mixture is incubated at room temperature for 1 minute to allow time for lysis and binding of plasmid DNA. Next, the closed end of the wells are pierced (illustrated in
In at least one embodiment, 400 uL of a second reagent is added to each well in the processing plate. An example second reagent is composed of the following reagents in the following proportions: 8.0 ml 1M Tris Acetate pH 7.0, 4.0 ml 2M Sodium Acetate, 200.0 ml IPA, 400.0 ul RnaseA, to 188.0 ml dH2O. The plate is incubated at room temperature for at least one minute. A vacuum is then applied, according to various embodiments of the present invention, to the closed end of the processing plate 3, while the open end of the processing plate is exposed to ambient pressure. The resulting pressure differential across the apertures 669, 671, and 673 forces the supernatant fluid, not shown, to flow through out of the wells through the aperture.
In various embodiments, 400 uL of the second reagent is again added to each well in the processing plate. The plate is incubated at room temperature for at least two minutes. A vacuum is then applied in a manner similar to the previous steps.
Next, 400 uL of a third reagent is added to each well in the processing plate. An example third reagent is composed of the following reagents in the following proportions: 8.0 ml 1M Tris Acetate pH 7.0, 4.0 ml 2M Sodium Acetate, 320.0 ml IPA, to 68.0 ml dH2O. Next a vacuum is applied for between 10 and 15 minutes to evacuate the reagents from the wells. In some embodiments, plasmid DNA is eluted to a collection plate by adding 120 uL of molecular grade water to each well, incubating for at least 3 minutes, locating the collection plate under the processing plate, and applying a vacuum to the closed end of the processing plate, while the open end of the processing plate is exposed to ambient pressure. The purified plasmid DNA is collected in the collection plate, according to some embodiments, in manners described elsewhere in this disclosure. In another example embodiment, purified DNA is collected by centrifuging the processing plate and collection plate combination at 2500 rpm for 1 minute.
In another example embodiment of the invention, a system and method for harvesting yeast plasmid DNA is provided. In one example embodiment, yeast cultures are incubated in a least one processing plate. Cells are harvested in the processing plate by centrifugation at 2500 g for at least 5 minutes. The supernatant is carefully poured off or pipetted out of the processing plate. Next, 150 uL of a first reagent is added to each well containing yeast cells in the processing plate. An example first reagent is composed of the following reagents in the following proportions: 200 nL β-mercaptoethanol to 800 uL lytic enzyme. The processing plate is vortexed for five seconds. Next the plate is incubated at 37 degrees centigrade for at least 60 minutes.
In at least one embodiment, 200 uL of a second reagent is added to each well in the processing plate. An example second reagent is composed of the following reagents in the following proportions: 295 g Guanidine isothiocyanate; 12.5 ml 1M Tris-HCL, pH 8.0; 5.0 ml 0.5 M EDTA; 25 ml 20% Sarkosyl; to 500 ml dH20. The processing plate it vortexed vigorously for one minute. Next, the mixture is incubated at room temperature for 1 minute to allow time for lysis and binding of plasmid DNA. Next, the closed end of the wells are pierced (illustrated in
In at least one embodiment, 400 uL of a third reagent is added to each well in the processing plate. An example third reagent is composed of the following reagents in the following proportions: 8.0 ml 1M Tris Acetate pH 7.0, 4.0 ml 2M Sodium Acetate, 200.0 ml IPA, 400.0 ul RnaseA, to 188.0 ml dH2O. The plate is incubated at room temperature for at least one minute. A vacuum is then applied, according to various embodiments of the present invention, to the closed end of the processing plate 3, while the open end of the processing plate is exposed to ambient pressure. The resulting pressure differential across the apertures 669, 671, and 673 forces the supernatant fluid, not shown, to flow through out of the wells through the aperture.
In various embodiments, 400 uL of the third reagent is again added to each well in the processing plate. The plate is incubated at room temperature for at least two minutes. A vacuum is then applied in a manner similar to the previous steps.
Next, 400 uL of a fourth reagent is added to each well in the processing plate. An example third reagent is composed of the following reagents in the following proportions: 8.0 ml 1M Tris Acetate pH 7.0, 4.0 ml 2M Sodium Acetate, 320.0 ml IPA, to 68.0 ml dH2O. Next a vacuum is applied for between 10 and 15 minutes to evacuate the reagents from the wells. In some embodiments, plasmid DNA is eluted to a collection plate by adding 120 uL of molecular grade water to each well, incubating for at least 3 minutes, locating the collection plate under the processing plate, and applying a vacuum to the closed end of the processing plate, while the open end of the processing plate is exposed to ambient pressure. The purified plasmid DNA is collected in the collection plate, according to some embodiments, in manners described elsewhere in this disclosure. In another example embodiment, purified DNA is collected by centrifuging the processing plate and collection plate combination at 2500 rpm for 1 minute.
The present invention provides methods and devices for preparing alternative substances from biological materials. The unique properties of these devices, which are described in detail in this disclosure, enable useful, novel methods for preparing a variety of substances. Specific substances that can be prepared from biological material by practicing the present invention include, but are not limited to: single and double stranded DNA molecules from bacteriophages; bacterial plasmids; fungal plasmids such as yeast plasmids; Bacterial Artificial Chromosomes (BAC's); viral nucleic acids, genomic DNA from a variety of cell types such as genomic DNA from nucleated blood cells; protein molecules; antibody molecules; RNA molecules; carbohydrate molecules; lipid molecules; and cell metabolites.
In addition, the present invention also provides novel methods and devices for processing biochemical samples. These methods and devices are particularly effective for enabling the preparation of biologically or biochemically derived molecules for biochemical manipulation or analysis. Examples of processes in which the methods and devices of the present invention are useful include, but are not limited to: nucleic acid template preparation for biochemical manipulations such as PCR or DNA sequencing; the clean-up of biochemical reaction products, such as DNA thermocycle sequencing products; the clean-up of PCR reaction products for further manipulation and/or analysis; the preparation of biochemically modified or processed protein molecules for further modification or analysis, such as preparation of protein fragments for analysis by MALDI-TOF mass spectrometry; and the preparation of labeled nucleic acid samples, such as cDNA labeled with fluorescent dyes for expression analysis with gene chips or spotted arrays.
A novel aspect of the present invention is the use of container piercing to change a reaction vessel from a vessel open at one point to a vessel with at least two apertures. As a result of the piercing process, the sample preparation vessel can be transformed from a container with certain utilities such as the ability to be used as a culture chamber for cell growth or as a collection vessel for centrifugation, to a modified container with a variety of alternative utilities, such as a filter device, a column for gel filtration or a column for chromatography. This change in functionality can occur without the need to transfer the material being processed from one vessel to another. Thus, this aspect of the invention provides a novel, useful mechanism to carry out a variety of new methods to prepare substances from biological materials and to prepare and purify biochemical samples for manipulation and analysis. It will be further apparent that the novel methods described here for processing samples in a single container will enable multiple processing steps to be combined and performed in parallel within the single container. This ability provides particular efficiency and utility.
The present invention provides methods and devices that fundamentally alter and improve these sample preparation processes in useful ways by allowing multiple, alternative processing steps, which otherwise would require multiple transfer steps to alternative containers, to be performed in a single container.
Specific examples of processes that can be performed in an improved way by employing the present invention, include, but are not limited to the preparation or purification of nucleic acids, proteins and other biologically derived macromolecules. The adaptation of existing methods to the alternative system provided by the present invention can be accomplished without the need for undue experimentation by appropriately configuring and implementing the methods and devices described in detail in this disclosure. To demonstrate the flexibility of the single container system for performing sample processing, several specific examples are provided below. It will be apparent that a variety of alternative methods can be enabled by practicing the present invention.
Deoxyribonucleic Acids. A variety of forms of deoxyribonucleic acid molecules can be isolated from biological materials using methods and devices provided by the present invention. For example, plasmid DNA molecules, bacteriophage M13, yeast plasmids, cosmids, or BAC's can be prepared from cells using the present invention. In a specific embodiment of the present invention, cells are grown in a cell culture block like the devices described herein, the cells being grown in the presence of a nucleic acid binding substrate such as silica particles. They are collected by centrifugation and resuspended in an aqueous buffer containing a chaotropic agent (with appropriate cell wall degrading enzymes being added in advance for organisms such as yeast, as needed) and sufficient salt concentration to allow DNA binding to the substrate. The culture block is then pierced to create filter columns and the binding substrate is washed with an appropriate wash buffer, such as a 50% isopropanol solution. It is desirable to add ribonuclease enzyme to the wash buffer to enzymatically degrade RNA molecules in the sample. This sample is further washed with an 80% isopropanol solution and then the binding substrate is dried such as by vacuum, followed by elution of the nucleic acid with a low salt solution, for example with water, and the nucleic acid is collected in a collection vessel. This can be performed, for example, by vacuum driven elution or by centrifugation.
Genomic DNA from whole blood. The methods and devices of the present invention are also useful to prepare genomic DNA from whole cells such as nucleated blood cells. Such methods are especially useful for genetic analysis, such as genotyping or SNP analysis. Whole blood can be added directly to a container such as described herein where the container has been loaded with an appropriate binding substrate for nucleic acid such as silica particles. The cellular material from the blood can then be collected by centrifugation and the liquid portion decanted away. The pelleted cells can be resuspended in an appropriate buffer for lysis and binding, for example a buffer with a chaotropic salt. The container is then pierced to create a filter column for further processing. The contaminating materials are washed away using appropriate wash buffers, such as appropriate salt containing buffers with 50% isopropanol. The sample is further washed with an 80% isopropanol salt containing buffer, dried, and the genomic DNA is eluted with a low salt elution buffer such as water, then collected, for example by centrifugation or vacuum elution into a collection vessel.
mRNA molecules. The isolation of mRNA molecules from cells is useful to analyze gene expression in a cell, for example by preparing fluorescently labeled cDNA from the mRNA and then hybridizing the cDNA to a DNA microarray. A biological material, such as mammalian cells from which RNA is to be isolated can be added directly to a device such as the 96 well block described herein. The block should also contain an mRNA specific binding matrix, for example an oligo dT containing cellulose resin. The chamber is pierced to create filter columns and washed with appropriate wash buffers to remove contaminants. The RNA is then eluted with an elution buffer such as water and collected in a collection vessel.
Antibody molecules. The manipulation of antibody molecules has been extensively employed to develop useful purification, analytical, and therapeutic processes. Thus detailed methods and protocols for the isolation of functional antibody molecules are well established. Appropriate antibody manipulation protocols can be adapted to use with the methods and devices of the present invention. For example, an antibody containing serum sample from an animal can be processed using the devices of the present invention by collecting the serum in closed block (processing plates) such as described herein, where the chambers of the block containing an appropriate antibody-binding substrate, such as a protein A or protein G containing resin to bind the selected antibody molecules to the substrate. The antibodies can then be further processed by piercing the vessels to create filter columns, rinsing these filter columns with wash buffers, and eluting the antibodies into a collection vessel with appropriate elution buffers.
Protein molecules. The isolation of specific protein molecules generally requires specific methods adapted to the properties of the individual protein to be isolated. This the particular steps to be followed will be chosen for the desired product. In general a biological sample will be prepared, for example by culturing cells in the 96 well culture block described herein. The cells will be collected by centrifugation and media decanted away. Then the cells will be resuspended in an appropriate resuspension, and lysis buffer. The isolation of the protein will proceed following piercing, using appropriate binding or chromatography resins within the chamber. In many cases it will be possible to specifically bind the desired protein using an antibody with specific affinity for the protein of interest. In this case the appropriate antibody would be attached to a suitable solid support using methods well known in the art. Alternatively, by configuring the processing chamber appropriately, for example by layering a chromatography resin on top of an ion exchange binding substrate, several alternative preparation processes can be performed on the protein within a single container.
It will be apparent to those skilled in the art that various other alternative processes can be enabled using the present invention.
While, for the purposes of disclosure there have been shown and described what are considered at present to be example embodiments of the present invention, it will be appreciated by those skilled in the art that other uses may be resorted to and changes may be made to the details of construction, combination of shapes, size or arrangement of the parts, or other characteristics without departing from the spirit and scope of the invention. It is therefore desired that the invention not be limited to these embodiments and it is intended that the appended claims cover all such modifications as fall within this spirit and scope.
Number | Date | Country | |
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Parent | 10677918 | Oct 2003 | US |
Child | 12455575 | US |