The present disclosure relates to a method of manufacturing a microfluidic device, which may precisely form a channel having a desired shape within one substrate using a wax regardless of a shape of a hydrophilic porous substrate, and more specifically, to a method of manufacturing a microfluidic device in which a microchannel is formed by a wax within one hydrophilic porous substrate, the method including: an operation of stacking and then heat-treating a transfer film on which a mirror image of a wax pattern is formed to form a microchannel and the substrate.

A microfluidic device and a detection method for the microfluidic device are provided. The microfluidic device includes a driving substrate configured to drive a movement of a droplet; and a position detector configured to detect a position of the droplet on the driving substrate.

The present invention relates to a sensor assembly (1) for body fluids. The sensor assembly (1) comprises: a measurement chamber (2) extending in an axial direction from an inlet end (3) to an outlet end (4), the measurement chamber having a transverse cross-section with side walls (5, 6) defining a chamber width in a horizontal direction, and with top and bottom walls (8, 7) defining a chamber height in a vertical direction, each of the side walls (5, 6), top wall (8) and bottom wall (7) having a respective wall wettability for aqueous solutions; a first sensor (10a-h) adapted to measure a first parameter of body fluids, the first sensor (10 a-h) having a first sensor surface (11a-h) exposed to the inside of the measurement chamber at a first axial position, the first sensor surface (11a-h) having a first wettability for aqueous solutions; and a second sensor (20) adapted to measure a second parameter of body fluids, the second sensor (20) having a second sensor surface (21) exposed to the inside of the measurement chamber (2) at a second axial position upstream or downstream from the first axial position, the second sensor surface (21) having a second wettability for aqueous solutions higher than the first wettability. At the second axial position, the chamber width exceeds the width of the second sensor surface (21), and the measurement chamber has a widening (22) in a horizontal direction as compared to the first axial position.

An example system includes an array of retaining features in a microfluidic cavity, an array of thermally controlled releasing features, and a controller coupled to each releasing feature in the array of releasing feature. Each retaining feature in the array of retaining features is to position capsules at a predetermined location, the capsules having a thermally degradable shell enclosing a biological reagent therein. Each releasing feature in the array of releasing features corresponds to a retaining feature and is to selectively cause degradation of the shell of a capsule. Each releasing feature is to generate thermal energy to facilitate degradation of the shell. The controller is to selectively activate at least one releasing feature in the array of thermally controlled releasing features to release the biological reagent in the capsules positioned at the retaining feature corresponding to the activated releasing feature.

An electrowetting device includes a first substrate, a plurality of first electrodes formed on the first substrate, a dielectric layer formed on the plurality of first electrodes, a first water-repellent layer formed on the dielectric layer, a second substrate, a second electrode formed on the second substrate, and a second water-repellent layer formed on the second electrode. The first substrate and the second substrate are arranged with a gap between the first water-repellent layer and the second water-repellent layer. The first electrode includes an indium oxide-zinc oxide layer, the dielectric layer includes a silicon nitride layer, and the silicon nitride layer is formed directly on the indium oxide-zinc oxide layer.

Provided herein is a method of concentrating a tethering complex in a region of an amphiphilic layer, such as a lipid membrane. Also provided herein are methods of assembling a tethering complex; methods of concentrating an analyte in the region of a detector; amphiphilic layers; and arrays and devices for use in the disclosed methods.

The invention is related to a device (1) for receiving a biological sample (3) wherein the device (1) comprises a plurality of wells (10) wherein each well (10) comprises an inner surface (14) facing a volume (60) for receiving a biological sample (3). The inner surface (14) comprises a top section (20) and a bottom section (30). The top section (20) and the bottom section (30) are connected via a circumferential step (40). The circumferential step (40) forms a stop for a tip of a pipette (70).

The present inventive concept relates to a microfluidic arrangement (1) for capillary driven fluidic connection between capillary flow channels (8, 16). The microfluidic arrangement (1) comprises: a first microfluidic system (4) comprising a first surface (5), and a first capillary flow channel (8), wherein the first capillary flow channel (8) has an elongation in a first plane, and the first surface comprises an outlet opening (9) in a plane different from the first plane, the outlet opening defining an outlet area (35) in the first surface and being adapted to allow fluidic communication with the first capillary flow channel thereby forming a flow outlet (12) of the first capillary flow channel, and a second microfluidic system (6) comprising a second surface (7) and a second capillary flow channel (16), wherein the second capillary flow channel (16) has an elongation in a second plane parallel to the first plane, and a portion of the second surface (7) comprises an inlet opening (13) in a plane different from the second plane, the inlet opening defining an inlet area (33) in the second surface and being adapted to allow fluidic communication with the second capillary flow channel thereby forming a flow inlet (20) of the second capillary flow channel, wherein the first microfluidic system (4) and the second microfluidic system (6) are arranged with the first and the second surfaces in contact such that the flow outlet (12) and the flow inlet (20) are interfaced, thereby allowing capillary driven fluidic connection between the first and the second capillary flow channels (8, 16), wherein the outlet area (35) overlaps at least a portion of the inlet area (33), said at least a portion of the inlet area (33) overlapped by the outlet area (35) being smaller than the outlet area (35).

A system for performing biological reactions is provided. The system includes a chip including a substrate and a plurality of reaction sites. The plurality of reaction sites are each configured to include a liquid sample of at most one nanoliter. Further, the system includes a control system configured to initiate biological reactions within the liquid samples. The system further includes a detection system configured to detect biological reactions on the chip. According to various embodiments, the chip includes at least 20000 reaction sites. In other embodiments, the chip includes at least 30000 reaction sites.

Tissue sample cassettes for receiving tissue samples include an upper tray including compartments separated by dividers, a lower tray coupled to the upper tray and having a central recess, and an absorbent material located in the recess of the lower tray. Related systems and methods for automated gross processing of tissue samples are also disclosed.