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 microdevice includes a first substrate; and a second substrate that is joined to the first substrate, and that includes at least one groove that forms at least one microchannel with the first substrate and recesses that form closed spaces with the first substrate. When viewed from above, the closed spaces are disposed sandwiching the least one microchannel.

Disclosed herein are finished products, methods, compositions and kits for derivatizing plastic (e.g., “polymer”) surfaces in a manner that renders the surfaces appropriate for various downstream applications. For example, flow cells incorporating modified plastic surfaces provide greatly enhanced stability for retention of attached chemical species such as polypeptides and nucleic acids.

A liquid storage and controlled-release device and a biological detection chip. The liquid storage and controlled-release device comprises a liquid storage capsule with a liquid storage body which is deformable under a pressure, and a sealing layer for sealing the liquid storage body. A support platform is provided right below the liquid storage capsule and tightly connected with the liquid storage capsule, wherein, a directional release chamber is provided at the middle of the support platform, and the directional release chamber is provided with a guiding chamber for collecting the liquid and a sharp edge for inducing break. Compared with the conventional technology, the opening for liquid release is at the end far away from the rotation center, so that the liquid can be released completely by the centrifugal force, ensuring the quantitative release of stored liquid and reducing the influence on the accuracy of the subsequent detection.

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).

Methods and devices for testing a biological sample are provided. A tape includes multiple channels or reservoirs having inlet and outlet ports. One tape having biological sample disposed in its channels is temporarily mated with another tape having reagents disposed in its channels via a serpentine belt and compression roller assembly. Pulsed fluidic operations combine the reagents and the biological sample for subsequent observation, detection, storage and/or disposal. Fluidic transfer is provided in a uniform operation or in conjunction with a sensory feedback assembly.

Devices and methods for controlling collection of liquid sample are described. In an example, a microfluidic device can include an analytical device and an actuator. The actuator can be connected to the analytical device. The actuator can be operable to absorb fluid. The actuator can guide the absorbed fluid to an input layer of the analytical device. The actuator can deform in response to an occurrence of an absorption condition. A degree of deformation of the actuator indicates a volume of fluid collected by the analytical device.

The present invention relates to encapsulated microfluidic packages and methods thereof. In particular embodiments, the package includes a device, a cradle configured to support the device, and a lid having a bonding surface configured to provide a fluidic seal between itself and the device and/or cradle. Other package configurations, as well as methods for making such fluidic seals, are described herein.

Methods and systems for processing polynucleotides (e.g., DNA) are disclosed. A processing region includes one or more surfaces (e.g., particle surfaces) modified with ligands that retain polynucleotides under a first set of conditions (e.g., temperature and pH) and release the polynucleotides under a second set of conditions (e.g., higher temperature and/or more basic pH). The processing region can be used to, for example, concentrate polynucleotides of a sample and/or separate inhibitors of amplification reactions from the polynucleotides. Microfluidic devices with a processing region are disclosed.

The disclosed microfluidic valves may include a valve body having at least one cavity therein, a gate transmission element separating the cavity into an input gate terminal and an output gate terminal, a gate port configured to convey drive fluid into the input gate terminal, and a fluid channel. The gate transmission element may include a flexible membrane and a plunger coupled to the flexible membrane. The gate transmission element may be configured to move within the cavity to inhibit a subject fluid flow from an inlet port to an outlet port of the fluid channel upon pressurization of the input gate terminal, and to allow subject fluid flow from the inlet port to the outlet port upon depressurization of the input gate terminal. Various other related systems and methods are also disclosed.