This invention relates generally to devices that measure properties of fluids within vessels, and particularly to microplates and carriers for handling test fluids.
In the field of cell analysis, cells are commonly placed in a multiwell microplate for purposes of testing multiple conditions and replicates in a single experiment. Standard microplates, such as 24- and 96-well plates, are two-dimensional arrays of wells. Such arrays include some wells that are at the border or edge of the array, i.e., in the first row, first column, last row, or last column. Border wells and non-border wells can experience different conditions; this is commonly known as an “edge effect”. Because such assays are typically conducted at mammalian body temperature (37° C.), and border wells are more exposed to the external environment, the environment within the border wells may be substantially different from that of the non-border wells. The evaporation of liquid from wells adjacent to the border of the plate occurs at a higher rate than that of non-border wells. This causes a temperature drop in the border wells due to evaporative cooling, resulting in an increase in the concentration of solutes in the liquid. Both the temperature differences and the concentration difference contribute to data inconsistency in these types of assays. Live-cell assays are particularly sensitive to these effects due to the dynamic nature of the assay and the sensitivity of living, metabolically active cells to the environmental conditions in which they are being measured. Examples of these types of assays include FLIPR calcium flux assays, Corning EPIC label-free assays, and certain high-content imaging assays.
Several solutions have been proposed and applied to such standard microplates to address this problem. One workaround is to sacrifice the use of the border wells in the assay. By simply filling them with fluid to the same height as the assay wells, the border wells provide a humidity buffer. This approach has serious drawbacks in that the capacity of the microplate is significantly diminished, and in the case of a 24-well plate more than half of the wells are sacrificed. As the size of the well array in the microplate decreases, a higher fraction of wells become border wells. At the extreme, in one-dimensional arrays, every well has a high rate of evaporation.
Another workaround is to seal the wells or plate by overlaying the assay wells with oil or wrapping the covered plate with a plastic paraffin film, such as Parafilm M® film available from Bemis Company, Inc., or similar material. One of the drawbacks to these methods is that gas exchange is reduced. Metabolically active cells require oxygen; thus restricting the supply of oxygen can be detrimental to the cells and cause changes in assay results.
Existing solutions to this problem include modifications to the instrumentation or the cell growth vessel, i.e., microplate and cover. A few instrumentation manufacturers attempt to mitigate these effects by putting humidity control into the measuring chambers in which the microplate is placed. In general, however, these options are rare as high humidity levels can cause problems with the instrument electronics.
Modifications to the cell growth vessel may include changes to the design of the microplate and lid. Changes to the lid include adding a moisture-holding layer to the lid. However, in the case of live-cell assays where addition of reagent during the course of the assay is required, a lid or cover cannot be used.
The addition of perimeter or border wells to the microplate provides an environmental buffer between the assay well and the ambient laboratory conditions. For example, a plate may have large edge troughs, e.g., four troughs, surrounding the array of wells. Fluid may be placed in each trough, thus providing an environmental buffer. A potential drawback of this design is the large volume of each trough. Because well plates are shallow, there is potential sloshing of the border fluid when the plate is tilted or moved around the laboratory. In addition, the depth of the troughs, being the same depth as that of the wells, may require that a significant amount of fluid, more than 10× the volume of the assay well, be added to each trough. Therefore the operator may need to use a different tool (such as a different volume pipet) to fill the border troughs and the assay wells.
Standard microplate designs include a lid or cover where the edge or skirt of the cover can be up to half the height of the plate itself and protrudes 1-2 millimeters (“mm”) beyond the wall of the plate. This may present a problem while handling these plates, as it takes some dexterity to consistently pick up both the plate and the lid off of a surface, e.g., to avoid accidentally picking up only the lid and thus exposing the contents of the plate. When dealing with cell cultures that must be maintained under sterile conditions, current plate and cover assembly designs introduce considerable risk to the integrity of the cultures. Similar risks apply to assays where the contents of the wells must be protected from ambient light.
Standard microplate designs have a fixed height and footprint, such that the volume of the wells varies with the number of wells arrayed in the plate. For example, a standard 384-well plate has four times as many wells as a standard 96-well plate, but each well is approximately one-fourth the volume. Likewise, as well density (i.e., wells per plate) goes down, the volume per well increases. This design, although convenient for maintaining a standard footprint, requires that the researcher use more cells and reagents per well when using a lower-density plate. In addition, the spacing between wells changes, which can be an inconvenience when adding reagents to the assay plate.
Presently, no microplate is commercially available for performing an assay on a fewer number of wells while maintaining standard volumes and well-to-well spacing. Maintaining these features and reducing the number of wells may require reducing the footprint. However, since many standard laboratory workflows and instruments are designed to this standard, an adapter or carrier of some sort would be required. Examples of instruments that accept standard-footprint microplates include plate readers, high content imaging systems, centrifuges, and automated plate handling robots.
Microscope slides adhere to a different standard in the lab, and some products exist that bridge the microplate and slide formats. Some commercially available slides contain assay wells fused to a glass microscope slide, providing assay wells with glass bottoms designed for high-resolution imaging on microscopes. Although they do provide wells, the dimensions of the wells vary and are not standard with respect to well-to-well spacing nor length and width dimensions.
A commercially available carrier for microscope slides that conforms to the Society for Laboratory Automation and Screening (“SLAS”) microplate footprint and height standards is designed for imaging applications, but the placement of the slides in the carrier allows for some variability in well position, which may make automated analysis challenging.
In an aspect, an embodiment of the invention may include a multiwell microplate for holding liquid samples. The multiwell microplate includes a frame defining a plurality of wells disposed in a single column, each well having an opening with a length l1; a moat disposed about the plurality of wells; and a plurality of walls traversing the moat. The walls define a plurality of compartments, each compartment having a length l2 selected from a range of greater than l1 and less than 6l1.
One or more of the following features may be included. The well length l1 may be selected from a range of 1 mm to 9 mm (0.04 to 0.35 in). The plurality of wells may include eight wells. The moat may include eight compartments.
Two compartments disposed on opposing sides of the single column of wells may be in fluidic communication via an equalizer channel. A depth of the two compartments in communication via the equalizer channel may be less than a depth of compartments adjacent thereto.
A depth of at least one compartment may be less than a depth of one of the wells, e.g., the depth of the at least one compartment may be up to 50% of the depth of one of the wells. A depth of a compartment proximate an end portion of the frame may be less than a depth of a compartment disposed at a center portion of the frame. All of the compartments may have a substantially equal length.
A lifting tab may be defined on an end portion of the frame. At least one well may be opaque white or opaque black. The frame may define an indent on a lower edge.
In another aspect, embodiments of the invention may include a multiwell microplate carrier including a body defining a plurality of regions configured to hold a plurality of multiwell microplates in parallel, each multiwell microplate defining a single column of wells, and each of the regions defining a plurality of openings adapted to mate with the single columns of wells.
One or more of the following features may be included. The body may have a base footprint with outside dimensions of approximately 5 inches by 3.4 inches. Each region may define eight openings. The body may define three or four regions configured to hold three or four multiwell microplates, respectively.
In yet another aspect, embodiments of the invention may include a cartridge for mating with the multiwell microplate described herein. The cartridge includes a substantially planar surface having a plurality of regions corresponding to a number of respective openings of the wells in the multiwall microplate. Also located in plural respective regions of the cartridge is a sensor or a portion of a sensor adapted to analyze a constituent in a well and/or an aperture adapted to receive a sensor. At least one port may be formed in the cartridge, the port being adapted to deliver a test fluid to a respective well of the plate. The multiwell microplate may include eight wells and the cartridge may include eight regions.
In still another aspect, embodiments of the invention include a method for preparing a liquid analytical sample. The method includes delivering the analytical sample to a well defined by a frame of a multiwell microplate. A fluid is delivered to a moat defined by the frame. The frame defines a plurality of wells disposed in a single column, each well having an opening with a length l1. The moat is disposed about the plurality of wells. A plurality of walls traverses the moat, the walls defining a plurality of compartments, each compartment having a length l2 selected from a range of greater than l1 and less than 6l1.
One or more of the following features may be included. Delivering the analytical sample to the well may include using a pipettor. Delivering the fluid to the moat may include using a pipettor.
Evaporation from peripheral wells of a multiwell microplate may have a negative impact on various analytical steps, including cell seeding, cell plate incubation and running assays. In particular, cell-based assays (“CBA”) with adherent cells are susceptible to edge effects from cell seeding and cell plate incubation. Live-cells assays such as label-free and extracellular flux (“XF”) measurements are also susceptible to edge effects during the running of the assays. Multiwell plate designs having moats with compartments to hold hydration fluid, e.g., water or cell media, at and/or near the edges of the multiwell plate, in accordance with embodiments of the invention, help reduce such edge effects, reducing the evaporation of fluid from the wells by providing a humidified buffer between the air above the wells and the drier air outside a perimeter of the plate.
Referring to
In one embodiment, the multiwell microplate 100 includes a one-dimensional pattern of wells complying, in relevant part, with the pattern and dimensions of a microplate, as described by the American National Standards Institute and Society for Laboratory Automation and Screening standards, including Height Dimensions for Microplates (ANSI/SLAS 2-2005, Oct. 13, 2011); Well Positions for Microplates (ANSI/SLAS 4/2004, Oct. 13, 2011); and Footprint Dimensions for Microplates (ANSI/SLAS 1-2004, Oct. 12, 2011), all incorporated by reference herein.
The multiwell microplate may be formed from a molded plastic, such as polystyrene, polypropylene, polycarbonate, or other suitable material. The bottoms of the wells may be transparent and the sides colored black to reduce optical cross-talk from one well to another. In some embodiments, e.g., for use with luminescence measurements, the wells may be white. In some embodiments, e.g., for use in high-resolution imaging applications, the plate may be formed with glass as the bottom of the wells and plastic polymer forming the sides of the plate and walls of the wells.
Each of the wells may have a top portion with an opening having a length l1 as well as a bottom portion that may be cylindrical or square, and may have a tapered sidewall. A seating surface may be provided to act as a positive stop for sensors disposed on barriers (see discussion of cartridge with respect to
A moat 130 extends about an external perimeter of the wells. A plurality of walls 140 traverse the moat, the walls 140 defining a plurality of compartments 150. The walls 140 are preferably thick enough to provide rigidity to the microplate, while being thin enough to be injection molded without distortion. Accordingly, a thickness of the walls may range from 0.5 to 1.5 mm, preferably about 1 mm. The compartments each have a length l2 that is preferably a multiple of l1 and less than 6l1, preferably about 2l1, and not less than 6 mm. For example, if a well opening has a length l1 of 9 mm, an abutting compartment may have a length of 2l1 of 18 mm. A length of less than 6 mm (9 mm well-to-well spacing) could make filling the compartments challenging. All of the compartments may have substantially equal longitudinal lengths, i.e., the length from one end wall to an opposing end wall varying no more than 25%.
In a preferred embodiment, the moat has eight compartments and eight wells, with one or more compartments having a length approximately equal to the sum of the lengths of approximately two well openings, plus a thickness of one or more walls defining the well openings.
Two compartments disposed on opposing sides of the single column of wells may be in fluidic communication via an equalizer channel 160. The moat may include two equalizer channels 160, one at each end of the multiwell microplate. To equalize the volumes of the compartments of the moat, a depth of two compartments in communication via the equalizer channel may be less than a depth of compartments adjacent thereto. In one preferred embodiment, the equalizer channel is disposed at an end of the multiwell microplate, and is 0.08 inches wide and 0.25 inches deep. The dimensions of the equalizer channel are preferably small enough to reduce the contribution of the channel width to the overall plate size but are wide enough to overcome surface tension and allow the chosen fluid to fill the channel. In a preferred embodiment, the channel has a feature 165 (e.g., surface tension breaker 165 as illustrated in
A depth of at least one compartment may be less than a depth of one of the wells, e.g., the depth of the at least one compartment may be 50% or less than the depth of one of the wells.
A depth of a compartment proximate an end portion of the frame may be less than a depth of a compartment disposed closer to a center portion of the frame. In one preferred embodiment, to maintain a constant fluid height across all compartments with 800 μl in end compartments connected by an equalizer channel and 400 μl of fluid in the inner compartments, the inner compartments may be 0.055 inches deeper than the outer compartments.
The moat may have a width of at least 0.2 inches and no more than 0.5 inches, preferably approximately 0.265 inches. A moat that is too narrow could minimize the benefit of having a hydrating barrier between the wells and the dry outside air; whereas, a moat that is too wide could introduce the risk of sloshing and contamination of the assay wells.
All of the compartments may be of substantially equal length, e.g., varying no more than 25%.
Various features of the moat facilitate its filling with a multi-channel pipettor design for Society for Biomolecular Screening (“SBS”) standard microplates. Suitable multi-channel pipettors include Eppendorf 3122000051 and Mettler-Toledo L8-200XLS+, available from Eppendorf AG and Mettler-Toledor International Inc., respectively. The walls defining compartments are positioned so as to not interfere with pipette tips on the multi-channel pipettor. Such multi-channel pipettors have a standard tip-to-tip spacing of 9 mm, so compartments of a moat preferably allow access of an equal number of pipet tips into each compartment. Equalizer channels at the ends allow fluid to be drawn from the side compartments, thereby enabling hydration fluids to surround the end wells. The compartments are preferably more than one well and less than six wells in length to reduce splashing of liquid out of the microwell plate or contamination of assay wells with hydration liquid. Finally, the moat depth is preferably 50% or less than the well depth to reduce the required volume of hydration liquid and to allow the use of a pipettor the same size as a cell pipettor.
A lifting tab 170 may defined on one or both end portions 190 of the frame. The lifting tab may have a length l3 of 0.3 to 0.55 inches, e.g., 0.435 inches. The lifting tab facilitates lifting of the multiwell microplate and a cover or a microplate and a cartridge, without removing the cover or cartridge.
The lower edge of the frame may define one or more indents 180. The indents may be positioned at the ends and/or the sides of the frame. The incorporation of one or more indents provides stability for the frame when positioned in a carrier tray. Moreover, without the indents, the frame would sit higher in the carrier, which may prevent its use in different instrumentation. The height of one multiwell microplate is preferably about 0.5 to 0.9 inches, more preferably 0.685 inches (17.4 mm) without the carrier. Side-loading plate readers, for example, have plate access heights of 16 mm to 28 mm. The indent allows placement of the plates in the carrier with minimal added height (0 to 0.05 inches, i.e., 0 to 1 mm) In one preferred embodiment, the carrier adds less than 0.001 inches to the height of the plate.
The relative surface areas of fluids in the compartments and the wells are relevant for the impact of the moat on reducing evaporation in the wells. If the surface area of the fluid in the compartments is too small, the reduction of evaporation in the wells may be negligible. If the surface area of the fluid in the compartments is larger than necessary for the desired impact, the multiwell microplate may be less compact than necessary, and may present a challenge in filling the compartments with the same pipettes that are used for filling the wells.
Preferred embodiments may provide the surface areas and volumes when fluid is introduced into the wells and compartments indicated in Table 1. Embodiments of the invention include ranges of the preferred values of at least ±25% and greater; preferably the ratios of volumes and surface areas of the wells and compartments are substantially equal to the indicated values, i.e., ±50%. In one preferred embodiment, the difference between the two bottom-up measurements in the compartments for the cell culture and assay conditions is 0.055 inches. This difference in depth results in the fluid height of all compartments being at a constant depth relative to the top surface of the plate (i.e., 0.180 inches). This difference compensates for the equalizer channel.
Cartridge
Referring to
Each of the ports 230 may have a cylindrical, conic or cubic shape, open at planar surface 205 at the top and closed at the bottom except for a small hole, i.e., a capillary aperture, typically centered within the bottom surface. The capillary aperture is adapted to retain test fluid in the port, e.g., by surface tension, absent an external force, such as a positive pressure differential force, a negative pressure differential force, or alternatively a centrifugal force. Each port may be fabricated from a polymer material that is impervious to test compounds, or from any other suitable solid material, e.g., aluminum. When configured for use with a multiwell microplate 100, the liquid volume contained by each port may range from 500 μl to as little as 2 μl, although volumes outside this range can be utilized.
Referring to
The cartridge 200 may be attached to the sensor sleeve, or may be located proximal to the sleeve without attachment, to allow independent movement. The cartridge 200 may include an array of compound storage and delivery ports assembled into a single unit and associated with a similar array of sensor sleeves.
Referring to
Cover
Referring to
Carrier Tray
Referring to
In one preferred embodiment, the carrier has three regions 510 defining a plurality of openings 520 configured to align and mate with the wells of each multiwell microplate 100. In one preferred embodiment, in use, the columns of wells of the multiwell microplates are disposed at positions that correspond to columns 3, 7, and 11 of a 96-well microplate. Since the wells of the disclosed multiwell microplates are located at positions defined by the ANSI/SLAS standard, no modification of the plate readers is required. A collar 530 surrounds the bottom region of each microplate well when installed in the cartridge. Each collar forms a circular opening that provides positioning as well as light blockage. The collar may be colored black to shield crosstalk light from fluorescent signaling molecules in wells, or may be white to amplify emitted light from luminescent markers. The carrier may include slots 540 that correspond to indents on the multiwell microplate. The skirts of two adjacent microplates may fit into each slot. Scalloped edges 550 enable a user to easily remove the microplates as necessary, while providing rigidity to the carrier.
In one preferred embodiment, the carrier openings allow the microplate to sit in the carrier at the same height as if the plate was not in the carrier, i.e., the height of the plate is equal to the height of the plate and carrier assembly.
Cartridges 200 and covers 400 may be placed over the microplates 100, as discussed above. The multiwell microplates and cartridges may generally be used as described in U.S. Pat. Nos. 7,276,351 and 8,658,349, incorporated by reference herein. Moreover, the individual wells, barriers, and ports may have any of the characteristics and features of the wells, barriers, and ports described in these patents.
In use, a liquid analytical sample may be prepared by delivering the analytical sample to a well defined by a frame of a multiwell microplate 100, and delivering a fluid to a moat 130 defined by the frame. The analytical sample may be, for example, cells in a media. The fluid may be the same media, or another liquid, such as water. Both the analytical sample and the fluid may be delivered by a pipettor; in some embodiments, the sample and the fluid may be delivered by the same pipettor.
Incubator evaporation experiments were run to compare evaporation in covered multiwell microplates with hydration fluid in moats and without such fluid. For each of six plates, 80 microliters of liquid was placed in each well, and for three of those plates, 400 microliters of liquid was placed in each compartment of the moat. Three multiwell microplates with covers but with no liquid in moats (“dry”) and three multiwell microplates with covers and with liquid in moats were incubated overnight in a humidified incubator at 37° C. in a 10% CO2 atmosphere. The volume of liquid remaining in each well was measured, and the following values determined.
Evaporation of liquid from wells in uncovered microwell plates was measured after conducting a mock assay (˜90 minutes) within an extracellular flux analyzer instrument. Referring to
Referring to
Referring to
Referring to
The invention may be embodied in other specific forms without departing from the spirit or essential characteristics thereof. The foregoing embodiments are therefore to be considered in all respects illustrative of the invention described herein. Various features and elements of the different embodiments can be used in different combinations and permutations, as will be apparent to those skilled in the art. Scope of the invention is thus indicated by the appended claims rather than by the foregoing description, and all changes which come within the meaning and range of equivalency of the claims are therefore intended to be embraced herein.
This application claims the benefit of priority to U.S. Provisional Application Ser. No. 62/006,593 filed Jun. 2, 2014, which is incorporated herein by reference in its entirety.
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Number | Date | Country | |
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20150343439 A1 | Dec 2015 | US |
Number | Date | Country | |
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62006593 | Jun 2014 | US |