An automated microfluidic bioreactor device and methods to rapidly detect drugs of abuse from human sweat are provided. The bioreactor can perform either single-plexed measurements (detecting only one target analyte at a time) or multiplexed measurement (detecting multiple analytes simultaneously). The bioreactor device has a cartridge comprising a capillary array that employs competitive enzyme-linked immunosorbent assay (ELISA) to detect the presence of various drugs or metabolite compounds. For example, four common drugs, methadone, methamphetamine, amphetamine, and tetrahydrocannabinol, were detected rapidly and quantitatively in about 16 minutes with a low sweat sample volume (about 4 μL per analyte) and a large dynamic range (methadone: 0.0016 ng/mL-1 ng/mL; METH: 0.016 ng/mL-25 ng/mL; amphetamine: 0.005 ng/mL-10 ng/mL; THC: 0.02 ng/mL-1000 ng/mL).

Devices that includes a first portion, the first portion including at least one fluid channel; a fluid actuator; an analysis sensor disposed within the fluid channel; a conductivity sensor disposed within the fluid channel; and an introducer; a second portion, the second portion comprising: at least one well, the well containing at least one material, wherein one of the first or second portion is moveable with respect to the other, wherein the introducer is configured to obtain at least a portion of the material from the at least one well and deliver it to the fluid channel, and wherein the fluid actuator is configured to move at least a portion of the material in the fluid channel.

An expandable array and methods of maintaining a biological sample within an expandable array are provided. The expandable array includes a plurality of receptacles configured to receive a biological sample and a plurality of beams comprising a programmable material. Each beam of the plurality of beams is located between and connects at least two receptacles. The programmable material can be a shape-memory polymer or a magnetoactive material that transitions the plurality of beams from an extended state to a contracted state upon application of a stimulus.

The subject of the invention relates to a tool for manipulating a plurality of plugs, taking the form of a comb (1) comprising: a body (7) provided with a row of teeth (4) having pointed distal portions (4p) spaced apart in a linear direction in order to engage with the cavities of the plugs; a system for separating the plugs from the teeth (4) that comprises a slide returned elastically and guided to slide with respect to the body (7) in a direction parallel to the direction of extension of the teeth, the slide being provided with the fingers of the comb, which are movable by sliding between the teeth (4), and a control (11a) accessible from a first portion (1a) of the comb and which, when pressed to move translationally, causes the fingers of the comb to slide in the direction of the pointed distal portions (4p) in order to eject the plugs from the teeth (4).

Disclosed herein is a multi-well plate for imaging small animals, which is designed so that a well is not shadowed at the edge thereof to be suitable for imaging of small animals. The multi-well plate for imaging small animals includes a plurality of wells each in the form of a groove formed on a plate body to store small animals, wherein each of the wells is gently slanted at a boundary with the plate body to form a groove in order to prevent the well from being shadowed at the boundary with the plate body when the well is captured from above by a camera and then imaged. Therefore, it is possible to accurately identify the positions of small animals since imaging is smoothly performed even if a small animal is located at the edge of each well.

The technology described herein generally relates to systems for extracting polynucleotides from multiple samples, particularly from biological samples, and additionally to systems that subsequently amplify and detect the extracted polynucleotides. The technology more particularly relates to microfluidic systems that carry out PCR on multiple samples of nucleotides of interest within microfluidic channels, and detect those nucleotides. The technology still more particularly relates to automated devices for carrying out pipetting operations, particularly on samples in parallel, consistent with sample preparation and delivery of PCR-ready nucleotide extracts to a cartridge wherein PCR is run.

A process for freeze drying a material. The process has the steps of (a) placing material to be freeze-dried in a vessel, the vessel comprising a container having a base, and at least one wall defining an opening at one end; (b) applying a membrane to the at least one wall to thereby cover the opening, wherein the membrane comprises an aperture which, in use, is aligned with the opening; and (c) subjecting the vessel to a lyophilisation procedure, wherein the membrane is in place on the container during the lyophilisation procedure.

Provided are devices, methods, and systems for temperature control of individual containers in a thermocycler for polynucleotide synthesis. Provided herein are devices, methods, and systems comprising a circuit patch having a heating element that is placed over a reaction container on a lid of the reaction container or directly over the reaction container Provided herein are devices, methods, and systems comprising a single-piece sensor assembly for a thermistor plate assembly comprising a sensor holder having a sensor pad that is in contact with the container holder.

The present invention is directed to a method of measuring cell migration by measuring the invasion ratio of cells incubated on a pillar array inserted into a well structure, the method including steps of: preparing a pillar array having a plurality of micropillars and a well structure having a plurality of microwells into which the plurality of micropillars is insertable, respectively; forming cell spheroids by incubating cells in an extracellular matrix attached to the end contact surfaces of the micropillars; allowing the cells contained in the cell spheroids to invade the end contact surfaces; staining and scanning the cell spheroids, the cells contained in the cell spheroids, and the cells that invaded the end contact surfaces; and calculating the invasion ratio of cells by the following equation through a fluorescence image of the scanned cells:

[00001]$\begin{array}{cc}\mathrm{Invasion}\mathrm{Ratio}=\frac{\mathrm{Invasion}\mathrm{cell}\mathrm{area}}{\mathrm{Total}\mathrm{cell}\mathrm{area}}=\frac{A_{\mathrm{Total}}-A_{\mathrm{spheroid}}}{A_{\mathrm{Total}}}& \left[\mathrm{Equation}\right]\end{array}$

wherein A.sub.total represents the total cell area, and A.sub.spheroid represents the spheroid area.

An elongated incubation trough has an indentation open toward a top end as well as a bottom. The indentation has a first receiving area to receive an elongated test strip as well as a second receiving area to receive an end section of a fluid line. The second receiving area is in fluidic communication with the first receiving area. A maximum width of the second receiving area at bottom height is greater than a maximum width of the first receiving area at bottom height.