An apparatus for capturing biological material. The apparatus includes: an optically readable capture particle (ORCP) including: one or more optically readable particles (ORPs) each including an optical barcode to identify the ORCP; and a plurality of biological capture sites associated with the one or more ORPs, each of the plurality of biological capture sites including a cellular barcode to identify the ORCP.

The invention relates to fused cyclooctyne compounds, and to a method for their preparation. The invention also relates to a conjugate wherein a fused cyclooctyne compound according to the invention is conjugated to a label, and to the use of these conjugates in bioorthogonal labeling, imaging and/or modification, such as for example surface modification, of a target molecule. The invention further relates to a method for the modification of a target molecule, wherein a conjugate according to the invention is reacted with a compound comprising a 1,3-dipole or a 1,3-(hetero)diene.

An object of a device and a method for detecting a substance to be measured according to an embodiment of the present disclosure is to conveniently detect a biological substance, such as a bacterium or a fungus. The detection device according to an embodiment of the present disclosure includes a container that retains a solution containing a substance to be measured and a magnetic labeling substance that binds specifically to the substance to be measured, a flow generating unit that generates a flow in a first direction at least in the solution, a magnetic field generating unit that generates a magnetic field gradient in the solution, and a detection unit that detects composite particles, based on motion of particles in a predetermined region in the solution, the composite particles including the substance to be measured and the magnetic labeling substance bound together.

Provided are: a coloring cellulose microparticle enabling false positive to be significantly reduced while maintaining a high detection sensitivity; and an immunochromatographic diagnostic kit using the same.

To provide a particle labeling reagent having low luminescent characteristics and improved water solubility.

Provided is a particle labeling reagent containing a compound represented by the following general formula (I-1) or (I-2).

##STR00001## (In the above general formula (I-1), p represents an integer of 1 to 3. In the above general formula (I-1), M represents a hydrogen atom or a mono- to tri-valent metal atom. In the above general formula (I-1), L.sup.1 represents a single bond or a (p+1)-valent group. In the above general formulas (I-1) and (I-2), L.sup.2 and L.sup.3 each independently represent a hydrogen atom or a photodegradable protecting group, and L.sup.2 and L.sup.3 may be the same or different. Provided that at least one of L.sup.2 and L.sup.3 represents a photodegradable protecting group. In the above general formula (I-2), L.sup.4 represents a monovalent group.)

Provided for herein is a polynucleotide-modified bioconjugate comprising a substrate such as an antibody or bead linked to a conjugate component via a nucleic acid linker. Also provided are methods of making and using such bioconjugates. Conjugation methods for creating the bioconjugate are stable, not chemically harsh, and efficient enough that post-conjugation purification may not be required. Further this disclosure provides for reducing the logistic overheads related to product lines by eliminating the need for many unique linkers per conjugation pair.

The present disclosure relates to a kit for detecting a soluble growth stimulation expressed gene 2 protein. In particular, the present disclosure relates to a latex-enhanced turbidimetric immunoassay kit for detecting the concentration and/or content of the sST2 in human samples. The kit can be used in transmission immunoturbidimetry and scattering immunoturbidimetry. The kit comprises a buffer system, an anti-interference component, latex microspheres, an anti-sST2 antibody, etc. The latex-enhanced immunoturbidimetric agent of the present disclosure can detect sST2 proteins within a range of <400 ng/ml in a sample, with a sensitivity of up to 0.1 ng/ml and a high specificity, accuracy and precision. The kit is suitable for a fully automatic biochemical analyzer and a scattering analyzer, and has the advantages of convenient and fast use and low cost, and can be used clinically to detect the sST2 protein.

An object of the present invention is to provide a kit, a method, and a reagent which prevent the problem of false positive due to nonspecific adsorption, suppress the increase in noise to be generated, and are capable of achieving high-precision measurement of a measurement target substance in a wide concentration range from a low concentration to a high concentration. According to the present invention, there is provided a kit for measuring a measurement target substance, the kit including: a first particle having a label and modified with a first binding substance capable of specifically binding to a measurement target substance; a second particle having no label and modified with a second binding substance incapable of specifically binding to the measurement target substance; a flow channel for flowing the first particle and the second particle; and a substrate having a third binding substance capable of specifically binding to the measurement target substance or a substance capable of binding to the first binding substance, in which the first particle having a label is a luminescent labeled particle containing at least one kind of compound represented by Formula (1) and a particle. ##STR00001## Each symbol in Formula (1) has the meaning described in the present specification.

Two or more upconverting particles are attached to each unit of one or more units of a chemical component in a sample, to form, for each unit of the chemical component, a multi-particle complex including the unit of the chemical component and two or more corresponding upconverting particles. The sample is illuminated by input light having a first wavelength. Light is received at an imaging sensor, the received light including output light generated by at least a portion of the upconverting particles attached to the units of the chemical component, the output light having a second wavelength that is shorter than the first wavelength. One or more images of the sample are captured from the received light. Based on the captured one or more images, a presence or a level of the chemical component in the sample is determined.

The present invention can be included in the field of diagnostics. The present invention provides hybridomas, antibodies and test devices for the detection of bacteria of the genus Campylobacterin a sample. Further, the present invention discloses the uses of the antibodies and a method for detecting bacteria of the genus Campylobacter. The antibodies of the present invention are specific for DNA-Binding Protein from Starved Cells (Dps) and provide less false positives and a higher sensitivity when used in an immunochromatographic test device than other antibodies used to detect bacteria of the genus Campylobacter.