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浆细胞瘤细胞核与细胞质中富含聚腺苷酸核糖核酸的测定。

Determination of polyadenylate-rich ribonucleic acid in the nucleus and in the cytoplasm of plasmacytoma cells.

作者信息

Abraham K A, Eikhom T S

出版信息

Biochem J. 1975 Sep;149(3):669-74. doi: 10.1042/bj1490669.

Abstract

A number of parameters affecting the adsorption of rRNA and poly(A)-containing RNA to Millipore filters were investigated separately. Binding of both types of RNA to the filter was dependent on the concentration of RNA, pH and Mg2+ concentration of the reaction mixture. Both types of RNA bound to the filter optimally at slightly acid pH values. The binding of poly(A)-containing RNA to the filter exhibited a broad pH-dependence compared with that of rRNA. The ratio of poly(A)-rich RNA/rRNA retained by the filter was maximal between pH7 and 8. The presence of 1 mM-EDTA or a high concentration of NaCl (over 0.5M) decreased the affinity of RNA for the filter. The amount of poly(A)-containing RNA in the nucleus and in the cytoplasm of a plasmacytoma cell line (MPC-11) labelled with [32P]Pi was determined by the Millipore-filter technique under conditions that minimized contamination by rRNA. These data were compared with the estimations made by oligo(dT)-cellulose chromatography. The results obtained by these two methods were in good agreement for RNA labelled for short periods (up to 2h). In long labelling and pulse-chase experiments, however, contamination of the filter by rRNA of increasing specific radioactivity in the cytoplasm gave an erroneous value for poly(A)-containing RNA by the Millipore-filter technique. Determinations made on the nuclear fraction by these two methods did not show significant variation in short- and long-term labelling experiments.

摘要

分别研究了影响rRNA和含多聚腺苷酸(poly(A))的RNA吸附到微孔滤膜上的多个参数。两种类型的RNA与滤膜的结合均取决于RNA的浓度、反应混合物的pH值和Mg2+浓度。两种类型的RNA在略酸性pH值下与滤膜的结合最为理想。与rRNA相比,含poly(A)的RNA与滤膜的结合表现出更广泛的pH依赖性。滤膜保留的富含poly(A)的RNA/rRNA比例在pH7至8之间最大。1 mM乙二胺四乙酸(EDTA)或高浓度氯化钠(超过0.5M)的存在会降低RNA与滤膜的亲和力。在将rRNA污染降至最低的条件下,采用微孔滤膜技术测定了用[32P]Pi标记的浆细胞瘤细胞系(MPC-11)细胞核和细胞质中含poly(A)的RNA的量。将这些数据与寡聚(dT)纤维素柱层析法的测定结果进行了比较。对于短时间(长达2小时)标记的RNA,这两种方法得到的结果吻合良好。然而,在长时间标记和脉冲追踪实验中,由于细胞质中比放射性不断增加的rRNA对滤膜的污染,使得微孔滤膜技术测定的含poly(A)的RNA值出现错误。在短期和长期标记实验中,用这两种方法对细胞核部分进行的测定未显示出显著差异。

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