A rapid sensitive method for the measurement of guanine ribonucleotides in bacterial and environmental extracts

A sensitive and rapid method has been developed for studying the interactions of ribonucleotide homopolymers with isolated liver ribosomal subunits. Small amounts of ribosomal subunits are first immobilised on Millipore filters. The homopolymers are then allowed to interact with the ribosomes by slo

PurgeIGC Cryogenic cooling Vinyl chloride ## Purgeable gases Nafion directly to a capillary column [4-71 cryogenic focusing is mandatory; otherwise, input bands for analytes become very broad over the 10-15 minute sample introduction time. For the most volatile compounds, such as the purgeable g

A protein assay is described in which the sample is precipitated with trichloroacetic acid in the presence of sodium dodecylsulfate, filtered off on a Millipore membrane and stained with Amidoschwarz 10B. The proteindye complex is eluted, and its absorbance determined at 630 nm. This assay is very r