A fluorescamine assay for submicrogram quantities of protein in the presence of Triton X-100

The Lowry procedure has been modified for use in the presence of Triton X-100 (TX-loo) by the addition of 10% sodium dodecyl sulfate. The method is applicable to samples containing 40-120 pg protein.

A procedure is described for the precipitation of protein from detergent-treated fractions of mammalian tissues. The protein in Triton X-100 and deoxycholatetreated fractions is precipitated by addition of sodium dodecyl sulfate in amounts nearly equivalent to that of the detergents, followed by tri

An automated assay for measuring nanogram and subnanogram quantities of protein in microliter samples was developed with the fluorometric reagent &phthaldialdehyde/mercaptoethanol. Low molecular weight interfering substances were separated within the analysis by gel filtration. The technique allowed

We report below on an extremely simple and somewhat more sensitive modification of the Chert procedure (1) for inorganic orthophosphate determination that has been routinely used in this laboratory for almost 2 years. The method overcomes the problem of precipitation of the phosphomolybdate complex

Fluorescamine is a useful reagent in monitoring protein-DNA interactions only if a convenient method of separating the complex from free protein is available. Sedimentation of the complex provides such a method at least in the case of histone-like proteins capable of extensive interaction with DNA.