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人血清和白细胞中酸性核糖核酸酶的纯化及性质

Purification and properties of acid ribonucleases in human serum and leukocytes.

作者信息

Akagi K, Yamanaka M, Murai K, Omae T

出版信息

Cancer Res. 1978 Jul;38(7):2163-7.

PMID:26464
Abstract

Acid RNase was purified from normal human serum about 2400-fold by chromatography on phosphocellulose and Sephadex G-75 and rechromatography on Sephadex G-75. Assayed with yeast RNA as substrate, the enzyme showed the maximal activity at about pH 6.5 with sodium phosphate buffer. The reaction was activated by Na+, K+, and spermine, but it was not affected greatly by Mg2+, Co2+, and EDTA. Ca2+, Fe2+, Zn2+, and Cu2+ inhibited the reaction. Among the synthetic substrates examined, the enzyme preferentially hydrolyzed pyrimidine nucleotides, with a higher affinity for polycytidylate than for polyuridylate. The enzyme was thermolabile, but it stabilized with bovine plasma albumin. The molecular weight was approximately 15,000, estimated gel filtration on Sephadex G-75, and its isoelectric pH was above 11.0. From normal human leukocytes, acid RNase was purified about 400-fold by the same procedure described previously except that rechromatography on Sephadex G-75 was omitted. The properties of leukocytic RNase were found to be similar to those of serum acid RNase, but the latter enzyme differed in substrate specificity substantially from leukocytic RNase, preferring polyuridylate to polycytidylate. This evidence shows that serum RNase is not of leukocytic origin under normal physiological conditions.

摘要

酸性核糖核酸酶通过磷酸纤维素和葡聚糖G - 75柱层析以及在葡聚糖G - 75上的再层析,从正常人血清中纯化了约2400倍。以酵母RNA为底物进行测定时,该酶在磷酸钠缓冲液中,pH约为6.5时显示出最大活性。反应被Na⁺、K⁺和精胺激活,但Mg²⁺、Co²⁺和EDTA对其影响不大。Ca²⁺、Fe²⁺、Zn²⁺和Cu²⁺抑制反应。在所检测的合成底物中,该酶优先水解嘧啶核苷酸,对聚胞苷酸的亲和力高于聚尿苷酸。该酶不耐热,但与牛血浆白蛋白一起时可稳定。通过葡聚糖G - 75凝胶过滤估计其分子量约为15,000,其等电点pH高于11.0。从正常人白细胞中,除了省略在葡聚糖G - 75上的再层析外,通过与先前所述相同的程序将酸性核糖核酸酶纯化了约400倍。发现白细胞核糖核酸酶的性质与血清酸性核糖核酸酶相似,但后者在底物特异性上与白细胞核糖核酸酶有很大不同,相对于聚胞苷酸更喜欢聚尿苷酸。这一证据表明,在正常生理条件下血清核糖核酸酶并非来源于白细胞。

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