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Purification and characterization of an endo-exonuclease from adult flies of Drosophila melanogaster.

机译:果蝇果蝇内切核酸外切酶的纯化和鉴定。

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摘要

An endo-exonuclease (designated nuclease III) has been purified to near homogeneity from adult flies of Drosophila melanogaster. The enzyme degrades single- and double-stranded DNA and RNA. It has a sedimentation co-efficient of 3.1S and a strokes radius of 27A The native form of the purified enzyme appears to be a monomer of 33,600 dalton. It has a pH optimum of 7-8.5 and requires Mg2+ or Mn2+ but not Ca2+ or Co2+ for its activity. The enzyme activity on double-stranded DNA was inhibited 50% by 30 mM NaCl, while its activity on single-stranded DNA required 100 mM NaCl for 50% inhibition. Under the latter conditions, its activity on double-stranded DNA was inhibited approximately 98%. The enzyme degrades DNA to complete acid soluble products which are a mixture of mono- and oligonucleotides with 5'-P and 3'-OH termini. Supercoiled DNA was converted by the enzyme to nicked and subsequently to linear forms in a stepwise fashion under the condition in which the enzyme works optimally on single-stranded DNA. The amino acid composition and amino acid sequencing of tryptic peptides from purified nuclease III is also reported.
机译:内切核酸外切酶(称为核酸酶III)已从果蝇果蝇的成年蝇中纯化至接近同质。该酶降解单链和双链DNA和RNA。它的沉淀系数为3.1S,冲程半径为27A。纯化后的酶的天然形式似乎是33,600道尔顿的单体。它的最佳pH值为7-8.5,并且需要Mg2 +或Mn2 +,但不需要Ca2 +或Co2 +来发挥作用。 30 mM NaCl可抑制50%的双链DNA酶活性,而50 m%抑制则需要100 mM NaCl的单链DNA酶活性。在后一种条件下,其对双链DNA的活性被抑制了约98%。该酶将DNA降解为完整的酸溶产物,该产物是具有5'-P和3'-OH末端的单核苷酸和寡核苷酸的混合物。在酶对单链DNA最佳作用的条件下,酶将超螺旋DNA逐步转化为切口,随后转化为线性形式。还报道了来自纯化的核酸酶III的胰蛋白酶消化肽的氨基酸组成和氨基酸测序。

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