Extraction of RNA from mammalian tissue culture cells

RNA extraction from mammalian tissue has been compared using the different deproteinizing agents: a) guanidine-HCl, b) guanidinium-thiocyanate, c) buffer-saturated phenol, or d) buffer-saturated phenol followed by a proteinase K digestion of the aqueous phase. Both solid tissues (first, second, and

A convenient and rapid procedure has been developed to extract RNA polymerase II quantitatively from cultured mammalian cells. The procedure was successfully employed on HeLa, CHO, L, and MDBK cells. The easy extraction of RNA polymerase II by freeze-thaw of cells in a buffer of low ionic strength s

A rapid procedure for the isolation of total RNA from small amounts of mammalian tissue (35 to 150 mg) is described. Tissues were homogenized in the presence of RNase inhibitors but in the absence of strong detergents. Contaminants were removed by phenol/chloroform extraction and Sephadex column chr