Agarosegelelectrophoresis
General ProcedureCast a gelPlace it in gel box in running bufferLoad samplesRun the gelImage the gelCasting Gels0.7% agarose gel with 1kbp ladder in UV and white light showing different dyesThe amount of agarose to use in your gel depends on the DNA in question. Use the following table as a rough guide:Agarose Concentration (g/100mL)Optimal DNA Resolution (kb)0.51 - 300.70.8 - 121.00.5 - 101.20.4 - 71.50.2 - 3Measure......阅读全文
DNA-mobility-in-gels
1. Migration of marker dyes in native polyacrylamide non-denaturing gels Gel % Bromophenol blue (BP) Xylene cyanole (XC) 3.5 100 460 5.0
Competitive-RTPCR-Strategy-for-Quantitative-Evaluation-5
3. Characterization of the method precision and repeatability.a. Ensemble PCRs in the same conditions established before using quantities of target in
Restriction-Digest
Materials:Restriction enzymes of choice, such as BamH1 and EcoRIRestriction enzyme reaction buffer, such as MULTI-CORE (TM) (Promega)70 % Ethanol100 %
RNAi实验中双链短RNA(dsRNA)制备过程
RNAi 实验中双链短RNA(dsRNA)制备过程,本实验方法来自于加州大学Jim教授实验,很权威!Procedure for the Generation of dsRNA for use in RNAi1. Design polymerase chain reaction (PCR ) prim
PCR产物纯化方法
Purification of PCR Products in Preparation for CloningJoseph SambrookPeter Maccallum Cancer Institute and The University of Melbourne, AustraliaDavid
DNA的酶学操作
DNA的酶学操作DNA Modifying Enzymes (Michael Blaber)Introduction to bacterial restriction/modification system. It provides very useful background knowledge
基于PCR技术的染色质沉淀分析1
INTRODUCTIONAfter chromatin immunoprecipitation (ChIP), different PCR-based approaches can be used to determine how much DNA is precipitated at a locu
基于PCR技术的染色质沉淀分析
INTRODUCTION After chromatin immunoprecipitation (ChIP), different PCR-based approaches can be used to determine how much DNA is precipitated at a loc
聚丙烯酰胺凝胶电泳(polyacrylamide-gel-electrophoresis,PAGE)
配制 Tris- 甘氨酸 SDS-PAGE 聚丙烯酰胺凝胶电泳分离胶所用溶液 溶液成分 不同体积( ml )凝胶液中各成分所需体积( ml ) 5 10 15 20 25 30 4
PCR的下游应用
· Agarose Gel Electrophoresis of PCR Products (Robert H. Cruickshank)· Agarose Gel Electrophoresis of PCR Products (Immunology Resourc
基因型分析
Randomly Amplified Polymorphic DNA (RAPD)Randomly Amplified Polymorphic DNA (RAPD) by (DNA KAFFE)RAPD analysis has been successfully used in mapping
PCR的下游应用
・ Agarose Gel Electrophoresis of PCR Products(Robert H. Cruickshank)・ Agarose Gel Electrophoresis of PCR Products(Immunology Resource)
Gene-splicing-and-mutagenesis-by-PCRdriven-overlap-extension
实验概要 Extension of overlapping gene segments by PCR is a simple, versatile technique for site-directed mutagenesis and gene splicing.Initial
Engineering-BioBrick-vectors-from-BioBrick-parts/Colony-PCR
MaterialsPCR SuperMix High FidelityVF2 primer (5''-TGCCACCTGACGTCTAAGAA-3'')VR primer (5''-ATTACCGCCTTTGAGTGAGC-3'')De
PCR实验指导与常见问题分析5
MgCl2 concentrationRelationship between MgCl2 and dNTP concentrationdNTP concentrations of about 200µM each are usually recommended for the Taq polyme
重组DNA的分离、克隆与测序实验手册8
B. Midiprep double-stranded DNA isolationA midi-prep double-stranded DNA isolation has been developed to generate a sufficient amount of template DNA
甲醛洋菜胶体电泳
甲醛洋菜胶体电泳 (formaldehyde-agarose gel electrophoresis)甲醛是一种常用的RNA 变性剂。在进行甲醛洋菜胶体电泳分析时,必须先配制含有甲醛的洋菜胶体,RNA 也必须先以甲醛及formamide 进行变性处理,以确保其二度结构充分被打开。由于甲醛可能是一种致
细胞支原体污染的PCR检测
支原体菌株来源: M.Arginini ATCC23838 精氨酸支原体 M.FermentaneATCC19989发酵支原体 M.SalivariumATCC23064唾液支原体 M.HominisATCC23114人型支原体 M.Ora
细胞支原体污染的PCR检测
支原体菌株来源:M.Arginini ATCC23838 精氨酸支原体M.FermentaneATCC19989 发酵支原体M.SalivariumATCC23064唾液支原体M.HominisATCC23114人型支原体M.OraleATCC23714口腔支原体M.HyorhinisATCC290
非变性胶蛋白电泳
Section 2.1Nondenaturing Polyacrylamide Gel Electrophoresis of ProteinsJohn M. Walker1. IntroductionSDS-PAGE (Section 2.2) is probably the most commo
DNA克隆
DNA克隆(主要内容如下)· General Procedure· PCR Cloning· Subcloning· ET Cloning· Vector Preparation· Ligation Re
Isoelectric-Focussing-of-Membrane-Proteins-by-Slab-Gel-Method
REFERENCE: Ames, G.F.L. and Nikaido, H. 1976. Biochemistry. 15:616-623.MATERIALS:Gel solution:1.05 gacrylamide0.032 gbis-acrylamide8.25 gurea6.5 mldis
Phage-DNA
IntroductionThe phage lysate from the plate contains bacterial DNA and RNA, as well as phage DNA encased in the phage coat. The following procedure, d
基于PCR技术的染色质沉淀分析
INTRODUCTIONAfter chromatin immunoprecipitation (ChIP), different PCR-based approaches can be used to determine how much DNA is precipitated at a locu
甲醛洋菜胶体电泳
实验概要本实验介绍了甲醛洋菜胶体电泳 (formaldehyde-agarose gel electrophoresis)的操作流程。实验原理甲醛是一种常用的RNA 变性剂,进行电泳时所使用的缓冲液为MOPS (3-[N-morpholino] propanesulfonic acid)。由于r
Competitive-RTPCR-Strategy-for-Quantitative-Evaluation-4
We have also been able to detect expression of this receptor in all studied tissues, which is consistent with the pleiotropic nature of growth hormone
TRFLP的优缺点
该技术在应用的过程中,肯定需要在实验条件上不断进行改进,而这种改进的好坏自然而然需要实验结果的验证。。V. Grüntzig在2002年做了该工作的一部分,结果认为,在限制性酶切时,很有必要去除其中影响DNA的酶切过程,并且实验证明了具体的酶切时间。具有说服力的结果如下: 1,T-RFLP出数据的
TRFLP技术的优缺点
T-RFLP(末端限制性片段长度多态性)该技术在应用的过程中,肯定需要在实验条件上不断进行改进,而这种改进的好坏自然而然需要实验结果的验证。V. Grüntzig在2002年做了该工作的一部分,结果认为,在限制性酶切时,很有必要去除其中影响DNA的酶切过程,并且实验证明了具体的酶切时间。具有说服力的
甲醛洋菜胶体电泳实验
甲醛洋菜胶体电泳 (formaldehyde-agarose gel electrophoresis)甲醛是一种常用的RNA 变性剂。用于(1)RNA的分离测定(2)RNA提纯。实验方法原理rRNA 占细胞RNA总量的80~85%,以ethidium bromide 染色后,呈现于胶体上的两个主要R
酵母人工染色体
· Easy YAC Preparation Method (Andrew Davies,Shaw lab)· Screening YAC libraries (Donis Keller Lab)This is a method for screening YAC l