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04716728001

Roche

重组DNase I,无RNase

from bovine pancreas, expressed in Pichia pastoris

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About This Item

EC 号:
3.1.21.1 (BRENDA, IUBMB)
UNSPSC代码:
12352204
NACRES:
NA.21
价格与库存信息目前不能提供

生物来源

bovine pancreas

质量水平

100

重组

expressed in Pichia pastoris

表单

solution

分子量

~39 kDa

包装

pkg of 10,000 U

制造商/商品名称

Roche

最佳pH

7.0-8.0

溶解性

water: soluble

相关类别

一般描述

重组DNase I是一种DNA特异性内切酶。该酶可通过水解连接到DNA上的磷酸二酯而催化双链及单链DNA的随机降解,形成寡核苷酸和单核苷酸的混合物。重组DNase I的生产过程中所使用的所有材料都无动物来源,因而可形成无动物源产物。

内容物
  • 重组DNasae I,不无RNase,10 U/μl
  • 孵育缓冲液,10x浓度

特异性

热灭活:一单位无RNase重组DNase I可在75 °C孵育10分钟进行热灭活。

重要提示:无RNase重组DNase I也可根据标准实验方案通过酚提取进行灭活并去除,分子生物学中的现有实验方案。

应用

在对RNase较为敏感的应用中,可采用无RNase的重组DNase I降解DNA。[1][2][3]例如,DNase I常用于:
  • 在RT-PCR之前去除RNA中的基因组DNA
  • 体外转录反应之后分离不含DNA的RNA
  • 进行缺口翻译
  • 在真核DNA中定位DNase敏感的区域

特点和优势

  • 可从任意RNA样品中去除DNA污染
  • 未检测出RNase或蛋白酶活性
  • 可热灭活,因而免去了有机提取的必要
  • 通过优化的孵育缓冲液进行运输,以最大限度维持DNase活性
  • 完全无动物来源过程生产,去除了动物来源材料相关的任何风险

包装

1个试剂盒包含2种组分

质量

杜绝污染:每批次都按照现有质检工艺检测以确保无RNase及蛋白酶。

产品规格

糖基化形式
重组DNase I异质性N端糖基化,因此会在电泳时呈现两条带。
二价离子要求
DNase I需要二价阳离子以实现最高活性。DNA特异性内切酶通过镁离子等离子激活,并由钙离子刺激。因此,酶会受到EDTA等金属螯合剂抑制。

单位定义

一单位指的在1ml的检测条件下可造成260 nm处吸光值提高0.001/min的酶活性。
反应条件:
根据以下检测混合物测定体积活性。将100 μg小牛胸腺DNA与40至70单位的无RNase重组DNase I在1x孵育缓冲液中+ 25°C下孵育。测定260nm处吸光度增量。

制备说明

激活剂:二价金属离子
工作溶液:储备溶液:20 mM Tris-HCl,50 mM NaCl,2 mM CaCl2,2 mM MgCl2,1mM二硫赤藓糖醇,0.1 mg/ml Pefabloc SC,50% 甘油(v/v),pH 7.6 (4 °C)。
孵育缓冲液(10x):400 mM Tris-HCl,100 mM NaCl,60 mM MgCl2 10 mM CaCl2,pH 7.9。
酶稀释液:25 mM Tris-HCl,50%甘油(v/v),pH 7.6 (4 °C)。

储存及稳定性

将未稀释的酶溶液-15至-25°C储存;缓冲液4°C储存。

其他说明

仅用于生命科学研究。不可用于诊断。

储存分类代码

12 - Non Combustible Liquids

WGK

WGK 1

闪点(°F)

does not flash

闪点(°C)

does not flash

历史批次信息供参考:

分析证书(COA)

Lot/Batch Number
50230600
40177200
28478600
14623600
14406200

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实验方案

DNase I Recombinant, RNase-free Protocol

DNase I from bovine pancreas is a glycoprotein of Mr 37000. A special procedure is used to remove RNases from the DNase preparation.

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