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Isoelectric focusing--polynucleotide/polyacrylamide-gel electrophoresis. A technique to separate and characterize nuclease activities.

机译:等电聚焦-多核苷酸/聚丙烯酰胺凝胶电泳。分离和表征核酸酶活性的技术。

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摘要

Individual native nuclease activities from human leucocytes are separated by using two-dimensional gel electrophoresis in an apparatus that allows the simultaneous running of 28 gels. Proteins are separated by isoelectric focusing in a disc gel, followed by electrophoresis into a slab gel containing DNA. Protein denaturants are avoided in the second dimension by the use of a running pH well above the optimal pH for DNAase (deoxyribonuclease) activity. Electrophoresed gels are incubated in appropriate buffers to activate nuclease activity. After staining for intact DNA, the positions of active enzymes, unobscured by the presence of other proteins, are revealed as colourless spots in a reddish-purple field. The technique is easy to use and is sensitive to 50pg of DNAase I. Versatility is provided by the use of either acidic or basic electrophoresis running buffers and by the use of specific gel incubation conditions to reveal different sets of enzyme activities. Two DNAases active at pH 7.4 in the presence of Mg2+ and Ca2+, and sixteen DNAases active at acidic pH and not requiring metals, are detected. Treatment of the human enzymes with specific glycosidases reveals that many of the human DNAases are glycoproteins containing negatively charged moieties and may be derived from modification of parent activities.
机译:来自人白细胞的单个天然核酸酶活性通过在允许同时运行28个凝胶的装置中使用二维凝胶电泳进行分离。通过在盘状凝胶中进行等电聚焦分离蛋白质,然后将其电泳成含有DNA的平板凝胶。在第二维中,通过使用远高于DNA酶(脱氧核糖核酸酶)活性最佳pH的运行pH可以避免蛋白质变性剂。电泳凝胶在适当的缓冲液中孵育以激活核酸酶活性。对完整的DNA染色后,在红紫色区域中,无色斑点显示了活性酶的位置,该位置未被其他蛋白质的存在所遮盖。该技术易于使用,并且对50pg的DNAase I敏感。通过使用酸性或碱性电泳运行缓冲液以及通过使用特定的凝胶温育条件揭示不同的酶活性,可以提供多功能性。在存在Mg2 +和Ca2 +的情况下,检测到两个在pH 7.4下有活性的DNAase,和在酸性pH下不需要金属的16个DNAase。用特定的糖苷酶处理人的酶后发现,许多人的DNA酶是含有带负电荷的部分的糖蛋白,可能来源于亲本活性的改变。

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