Translation of "Receptor assay" in German

In the further preferred embodiment of the agglutination assay receptor R1 is a particle coated with one of the two defined antibodies while the other receptor is a particle coated with the other antibody.

The method according to the invention is carried out according to the principle of a ligand receptor assay i.e. an analyte present in the sample liquid is detected qualitatively or/and quantitatively by binding to a labelled receptor.

The present invention in addition concerns a reagent for the detection of an analyte in a sample liquid according to the principle of a ligand receptor assay characterized in that it contains a dispersion of gaseous, liquid or/and solid components in a liquid which effect a randomization of the light generated in the luminescent reaction and if desired the formation of a preferential direction in the light scattering.

Finally the invention also concerns a reagent kit for the detection of an analyte in a sample liquid according to the principle of a ligand receptor assay comprising a reagent according to the invention and a receptor spatially separated therefrom which carries a luminescent label.

The compounds were examined with membranes of recombinant CHO-ORL 1 cells in a receptor binding assay with 3 H-nociceptine/orphanin FQ.

The compounds were examined with membranes of recombinant CHO-ORL 1 cells in a receptor binding assay with 3 H-nociceptin/orphanin FQ.

The 4-aminocyclohexanol derivatives of the general formula I were investigated in a receptor binding assay with 3 H-nociceptin/orphanin FQ with membranes of recombinant CHO—ORL1 cells.

The cyclohexane derivatives of general formula I were examined in a receptor binding assay with 3H-nociceptin/orphanin FQ with membranes of recombinant CHO-ORL1 cells.

The compounds were examined with membranes of recombinant CHO—ORL 1 cells in a receptor binding assay with 3 H-nociceptin/orphanin FQ.

The compounds were investigated in a receptor binding assay with 3 H-nociceptin/orphanin FQ with membranes from recombinant CHO-ORL1 cells.

The cyclohexane derivatives of the general formula I were investigated in a receptor binding assay with 3 H-nociceptin/orphanin FQ with membranes from recombinant CHO-ORL1 cells.

As an example for the determination of the concentration of GnRH receptors on cell membrane extracts of cell lines and/or cell cultures, the Decapeptyl® radio receptor assay is used with membranes (as described by Emons, G., et al., 1993, Cancer Research 53, 5439-5446).

The cyclohexane compounds of the general formula I were investigated in a receptor binding assay with 3 H-nociceptin/Orphanin FQ with membranes of recombinant CHO-ORL1 cells.

The cyclohexane derivatives of the general formula I were investigated in a receptor binding assay with 3 H-nociceptin/orphanin FQ with membranes of recombinant CHO-ORL1 cells.

The cyclohexane-1,4-diamine compounds of the general formula I were investigated in a receptor binding assay with 3 H-nociceptinlorphanin FQ with membranes of recombinant CHO-ORL1 cells.

The cyclohexane-1,4-diamine compounds of the general formula I were investigated in a receptor binding assay with 3 H-nociceptin/orphanin FQ with membranes of recombinant CHO-ORL1 cells.

The cyclohexane-1,4-diamine compounds corresponding to the formula I were investigated in a receptor binding assay with 3 H-nociceptin/orphanin FQ with membranes of recombinant CHO-ORL1 cells.

The 4-alkyl-/4-alkenyl-/4-alkynylmethyl/-1-aryl-cyclohexylamine compounds corresponding to formula I were examined in a receptor-binding assay with 3 H-nociceptin/orphanin FQ with membranes of recombinant CHO-ORL1 cells.

The advantage of the use of a reporter protein which is broken down faster in an assay cell is obvious in the light of fact that a low background expression of the reporter gene construct will virtually always be detectable under the assay conditions, even without activation of the Ras or Ras-like signal pathway through the membrane receptor in the assay cell: the fast breakdown of the reporter protein significantly reduces the signal resulting from this background expression on detection of the protein level, i.e. of the reporter protein, because there is no accumulation of reporter protein over time.