Übersetzung für "Assay buffer" in Deutsch

The remaining reaction mixture is removed by suction and the magnetic particles are washed with assay buffer.

The measuring chamber is filled with assay buffer and the measured signal is recorded.

The conjugate and the antiserum dilutions were prepared with assay buffer.

The manufacturer's assay buffer 1 without addition of protein is used as the negative control.

An assay buffer which had the following composition was used for the determinations:

This is the measurement in the absence of substance, measured in sodium-free transport assay buffer.

This is the measurement in the absence of substance, measured in sodium-containing transport assay buffer.

The assay buffer (pH 7.4) has the following composition (per liter): tris 6.057 g;

Like our previous formulation, the new HRP-Protector™ is also a very good assay buffer.

Blank control: assay buffer with 1% DMSO was added to the dilution series of the microtiter plates as a blank control.

The assay buffer was removed and each well was washed five times with in each case 200 ?l washing buffer.

200 ?l of a 1:1000 dilution of the above tracer concentrate in assay buffer were then pipetted into each tube.

The secreted receptor proteins are directly used in the assay in the form of certain dilutions in the assay buffer.

For the detection reaction, reconstitution of the lyophilized components takes place by dissolution in an assay buffer.

For the leakage assay at various pH values, the liposome stock solution was diluted (6 ?l/ml) in 2× assay buffer (400 mM NaCl, 40 mM Na titrate).

Fresh human erythrocytes were washed with HBS several times and resuspended in 2× assay buffer of the appropriate pH (300 mM NaCl, 30 mM Na titrate) at a concentration of 6.6 107 /ml.

For the leakage assay at various pH values, the liposome stock solution was diluted (6 ?l/ml) in 2 x assay buffer (400 mM NaCl, 40 mM Na citrate).

Fresh human erythrocytes were washed with HBS several times and resuspended in 2× assay buffer of the appropriate pH (300 mM NaCl, 30 mM Na citrate) at a concentration of 6.6 107 /ml.

Fresh human erythrocytes were washed with HBS several times and resuspended in 2 x assay buffer of the appropriate pH (300 mM NaCl, 30 mM Na citrate) at a concentration of 6.6 10 7 /ml.

For this purpose 25 ?l clear result was transferred to a glass test tube (or into a special-RIA-container from Sarstedt, Darmstadt) and 10 ?l tracer (3 H-25-OH-D), 300 ?l assay buffer and 100 ?l vitamin D-binding protein (not in NSB) added.

For determination of the calibration curve or as standard, there were employed solutions of 1,25-dihydroxy vitamin D in assay buffer with the following concentration: 0, 6.6, 20, 60 and 180 pg/ml (see calibration curve in FIG. 5 C).

For the assay buffer, 5 g casein was dissolved in 100 ml 0.1 N NaOH and topped up with PBS, pH 7.4 to 1 L volume.