核酸内切酶
- 名endonuclease
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核酸内切酶在DNA断裂损伤检测中的应用研究
Application of Endonuclease to Detecting the Strand Breaks of DNA Oxidative Damage
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限制性核酸内切酶与DNA相互作用研究进展
Progress on the Interaction of Restriction Endonuclease and DNA
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补充核酸内切酶Ⅲ对DNA氧化损伤影响的研究
The effect of endonuclease ⅲ supplementation on the damage of DNA strand breaks
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人乳头瘤病毒DNA的限制性核酸内切酶分析
Restriction enzyme analysis of human papilloma virus ( hpv ) dna from common warts
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该法提取的血吸虫基因组DNA较纯,适合于以后进行DNA限制性核酸内切酶谱分析和Southernblot分析。
The technique is useful in the analysis of restriction endonuclease digestion of genomic DNA and Southern blot .
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本文应用限制性核酸内切酶HaeⅢ显示了孟氏裂头绦虫染色体G分带,获得了较好的G带带纹。
G-banding of the chromosomes meets with success by using restriction endo-nucleas Hae ⅲ in Spirometra mansoni .
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T4核酸内切酶V的分离纯化
Isolation and Purification of T4 Endonuclease V
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HSV临床分离株的限制性核酸内切酶酶切分析与鉴定
Restriction endonuclease cleavage analysis of DNAs from herpes simplex verus clinical isolates
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方法:用甲基化敏感的限制性核酸内切酶消化,结合聚合酶链反应(PCR)技术。
Methods : 20 cases of MDS patients were studied using methylation sensitive restriction enzyme digestion and polymerase chain reaction ( PCR ) technique .
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结果:PCR和限制性核酸内切酶图谱分析均证实所获重组质粒中含有P1蛋白基因。
Results : Recombinant plasmid was proved to carry P1 protein gene by using PCR and endonuclease map analysis method .
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限制性核酸内切酶PstⅠ活性基团的研究
Studies on the Active Groups of Pst I Restriction Endonuclease
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方法应用PCR技术扩增T细胞受体γ链基因重排,选用四种限制性核酸内切酶消化扩增产物。
Methods After amplifying T-cell receptor γ chain gene rearrangement using polymerase chain reaction ( PCR ), we digested the products with 4 kinds of restriction enzyme .
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目的研究人胃黏膜上皮细胞系无嘌呤无嘧啶核酸内切酶(APE)的表达状况。
Objective To study the expression of APE / Ref-1 in gastric mucosal epithelial cell lines .
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Ⅱ型限制性核酸内切酶NcrⅠ的研究
Study on A Type ⅱ Restriction Endonuclease Ncr ⅰ
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Serratiamarcescens非特异性核酸内切酶的原核表达及其应用
Prokaryotic Expression and Application of Serratia marcescens Non-specific Endonuclease
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结果:(1)通过DNA测序和限制性核酸内切酶酶切鉴定证实,hMMP-12成功克隆到所需表达载体中;
Results : ( 1 ) The hMMP-12 was successfully cloned into the needed vector by enzymatic digestion and DNA sequencing ;
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以DNA分子与各种生化酶(Nicking核酸内切酶、核酸外切酶、聚合酶)间的生化反应来模拟数据的读取和写入。
Biochemical reactions between DNA memory and enzymes ( Nicking Endonuclease , Exonuclease and Polymerase ) can be defined as reading and writing operations .
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质粒pBR322的体外扩建以及有关限制性核酸内切酶图谱
In vitro Enlargement of pBR322 and the Related Restriction Enzyme Maps
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通过PCR扩增狂犬病病毒SAD-B19株的G、N基因。将回收的目的片段用限制性核酸内切酶PstI进行酶切。
The G and N gene of rabies virus SAD-B19 strain were amplified by PCR , the target genes were collected and digested by Confine digestion enzyme of PstI .
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在没有核酸内切酶存在时,QDs的荧光通过能量转移被猝灭,纳米探针处于关闭状态。
In the absence of endonucleases , the fluorescence of QDs is quenched through energy transfer effect , and the nanoprobe stays in the " OFF " state .
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目的:观察脑缺血后半胱氨酸蛋白酶3(caspase-3)和脱嘌呤/脱嘧啶核酸内切酶(APE/Ref-1)的表达,探讨脑缺血损伤与修复机制。
AIM : To explore the mechanism of neuronal injury and repair by investigating the expression of caspase-3 and apurinic / apyrimidinic endonuclease ( APE / Ref-1 ) after focal cerebral ischemia .
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目的氧化/还原因子1(ref1),也称为AP核酸内切酶(APE),是氧化还原和DNA碱基切除修复途径中的重要一员。
Objective Redox factor 1 ( ref-1 ), also known as AP endonuclease ( APE ), is one of the very important components of DNA base excision repair and redox .
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目的探讨DNA损伤修复基因脱嘌呤/脱嘧啶核酸内切酶(APE1)在鼻腔NK/T淋巴瘤中的表达及其临床意义。
Objective To investigate the expression of DNA damage and repair gene Apurinic / apyrimidinic endonuclease ( APE1 ) protein in nasal NK / T cell lymphoma , and elucidate its clinical implication .
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T7核酸内切酶I(T7EndonucleaseI,T7EndoI)是一种研究非常深入的多功能核酸内切酶,由大肠杆菌T7噬菌体基因3编码。
T7 Endonuclease I ( T7 Endo I ) is a very in-depth studied multi-functional endonuclease , which is coded by Escherichia coli T7 phage gene 3 .
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用X-gal平板及质粒图谱分析方法筛选重组克隆株,再用限制性核酸内切酶酶切图谱分析鉴定。
The recombinant clone was screened by X-gal plate and plasmid map , and identified by restricted enzyme mapping analysis method .
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方法应用聚合酶链反应、DNA测序和限制性核酸内切酶酶切等技术对15个AR-JP家系先证者的parkin基因进行突变研究。
Methods the polymerase chain reaction ( PCR ), DNA sequence analysis , and restriction enzyme digestion analysis were applied to check parkin gene mutations of 15 index patients from 15 families with AR-JP .
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由此可见,抗APO-1单抗与其特异性抗体结合后可能是通过使胞浆中游离Ca2+浓度升高,激活了Ca2+/Mg2+依赖的内源性核酸内切酶而导致SEB活化的淋巴细胞凋亡。
It suggests that the Ca 2 + / Mg 2 + depended nucleic acid endonuclease in lymphocytes treated with SEB is activated when APO 1 receptors on cells interact with its specific antibody and induce activated lymphocytes apoptosis finally .
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其特点在于结合使用限制性核酸内切酶EcorI及纳米金标记的检测探针,能够很好的降低背景值并有效增强信号。
It features combined with restriction endonuclease ECoR I and nano-gold-labeled detection probe that can reduce the background of a very good value and effective way to boost the signal .
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GzmA靶向作用于一种与内质网结合的特殊的复合体&SET复合体,其包含3种GzmA底物:核小体装配蛋白SET、DNA结合蛋白HMG-2、具有碱基切除修复作用的核酸内切酶Apel。
A special target of the granzyme A cell death pathway is an endoplasmic reticulum-associated complex , called the SET complex , which contains three granzyme A substrates , the nucleosome assembly protein SET , the DNA-binding protein HMG-2 , and the base excision repair endonuclease Apel .
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利用限制性核酸内切酶PstⅠ在不同的有机介质中的催化反应,研究了水含量、相对粘度,介电常数和渗透压等介质的物化性质对PstⅠ原活性和星号活性的影响。
Through the catalyzed reactions of the restriction endonuclease Pst ⅰ in different organic medium , the effect of the four physico-chemical properties such as total water content , relative viscosity , dielectric constant and osmotic pressure on the prime and the star activity of Pst ⅰ was studied .