An immunoassay includes forming first mixtures by reacting a combination reagent with serum of a subject; simultaneously forming second mixtures by reacting randomly selected platelet samples with the serum wherein in each mixture there are immunity compounds formed by combining the platelet antigens with predetermined antibodies in the serum, and other platelet antigens and other antibodies in the serum not forming the immunity compounds; preparing an interception device including receptacles and a filter net; placing each mixture in one receptacle; washing the mixtures wherein the mixtures forming the immunity compounds are intercepted by the filter net with others passing through; adding a signal sensing reagent to each receptacle; reacting the signal sensing reagent with the intercepted mixtures forming the immunity compounds to form final products; and performing a signal sensing to determine whether the final products contain anti-platelet antibodies and determine compatibility of cross matching of respective platelet samples.

A biosensor system for the detection of target analytes that includes a living biological cell of a predetermined type; a signal-generating reporter associated with the living biological cell; a signal transduction pathway or other activator mechanism or means associated with the signal-generating reporter; a universal detector element associated with the activator mechanism; and an analyte binding element associated with the universal detector element, wherein the analyte binding element is specific to both the universal detector element and a target analyte.

A biosensor system for the detection of target analytes that includes a living biological cell of a predetermined type; a signal-generating reporter associated with the living biological cell; a signal transduction pathway or other activator mechanism or means associated with the signal-generating reporter; a universal detector element associated with the activator mechanism; and an analyte binding element associated with the universal detector element, wherein the analyte binding element is specific to both the universal detector element and a target analyte.

The present invention relates to chimeric receptors that can be used in whole-cell sensors for detecting analytes of interest. The inventors showed that the DNA binding domains and downstream gene expression can be activated via dimerization of an artificial dimerization composed of a single chain variable domain. They demonstrated for the first time that an artificial bacterial receptor using an antibody-like domain can be activated and produce a transcriptional output upon ligand-binding. In particular, the present invention relates to a chimeric receptor polypeptide comprising: i) a first DNA binding domain, ii) at least one binding domain selected from the group consisting of heavy chain variable domain, camelid VHHs, or antibody mimetics having specificity for an analyte, and iii) a linker between the DNA binding domain and the binding domain.

The present invention relates to use of an Anaplasma phagocytophilum protein APH1384 as diagnostic antigen for granulocytic anaplasmosis. The protein can remedy the drawback of missed detection of an existing diagnostic antigen P44 for granulocytic anaplasmosis, improve sensitivity of detection for granulocytic anaplasmosis, and facilitate rapid and accurate clinical diagnosis of granulocytic anaplasmosis.

The present invention provides an improvement method and a system for decreasing the limit of detection of the presence of an analyte in a sample. In particular, the present invention provides an article or a system, such as a diagnostic kit, for detecting the presence of an analyte in a sample, comprising (i) a microsphere coated with an affinity ligand, or a spore or bacterium expressing one or more proteins on the surface thereof, (ii) a signal-producing substances, and (iii) a binding agent, wherein the signal-producing substance is conjugated with the binding agent and an antibody specific to the affinity ligand on the microsphere or the protein expressed by the spore or bacterium, wherein the signal-producing substances are conjugated to the microsphere, spore or bacterium through the binding of the antibodies specific to the affinity ligand or the protein.

The present invention provides an improvement method and a system for decreasing the limit of detection of the presence of an analyte in a sample. In particular, the present invention provides an article or a system, such as a diagnostic kit, for detecting the presence of an analyte in a sample, comprising (i) a microsphere coated with an affinity ligand, or a spore or bacterium expressing one or more proteins on the surface thereof, (ii) a signal-producing substances, and (iii) a binding agent, wherein the signal-producing substance is conjugated with the binding agent and an antibody specific to the affinity ligand on the microsphere or the protein expressed by the spore or bacterium, wherein the signal-producing substances are conjugated to the microsphere, spore or bacterium through the binding of the antibodies specific to the affinity ligand or the protein.

A system for use in rapid sample analysis that includes a biosensor reagent, wherein the biosensor reagent includes living biological cells; a reservoir card, wherein the reservoir card stores the biosensor reagent; and a test cartridge base, wherein the test cartridge base is configured to accept the reservoir card, and wherein the test cartridge base further includes a reaction chamber having a central axis, wherein the reaction chamber has the shape of a revolved half ellipse; an inlet channel connected to the reaction chamber, wherein the inlet channel is positioned above the reaction chamber at an angle of 15-60 degrees above the horizontal, and wherein the inlet channel is offset from the central axis of the reaction chamber; and a temperature control system for controlling the temperature of the biosensor reagent, the reservoir card, the test cartridge base, the reaction chamber, and the inlet channel individually or in various combinations.

Described herein are materials and methods of incorporating CLIP peptide into the peptide binding groove of HLA Class II antigens and using such HLA Class II antigens for the detection of alloantibodies.

Described herein are materials and methods of incorporating CLIP peptide into the peptide binding groove of HLA Class II antigens and using such HLA Class II antigens for the detection of alloantibodies.