PreparationofAgaroseGelsforDNAseparations
Weigh out the desired amount of agarose and place in an Erlenmeyer flask with a measured amount of electrophoresis buffer, e.g. for an 0.8% gel, add 0.8 gm of agarose and 100ml of TBE Buffer (1X), to a 200 ml flask. The larger flask insures against the agarose boiling over. Dissolve the agarose in a boiling water bath or in a revolving-plate microwave oven. All the grains of agarose should be dissolved and ......阅读全文
Preparation-of-Agarose-Gels-for-DNA-separations
Weigh out the desired amount of agarose and place in an Erlenmeyer flask with a measured amount of electrophoresis buffer, e.g. for an 0.8% gel, add 0
ELECTROPHORESIS-OF-DNA-IN-AGAROSE-GELS
ELECTROPHORESIS OF DNA IN AGAROSE GELSA). AGAROSE CONCENTRATIONS: Use 0.8% agarose (w/v) for high molecular weight DNA fragments, and 1 - 1.2% f
Agarose-Gels-for-Single-Stranded-DNA
1. Prepare 50X TAE as:242 g Tris Base57.1 mL Glacial Acetic Acid100 mL 500 mM EDTA, pH 8.0600 mL ddH2OMix. Bring volume to 1 L. Autoclave.2. Mix the f
DNA-Purification-from-Agarose-Gels
1. Separate DNA fragments in an agarose gel cast with 0.5 mg/mL Ethidium bromide. Locate bands with a hand-held long-wave UV lamp.2. Slice the gel wit
Preparation-of-Yeast-DNA-Embedded-in-Agarose-Plugs
Preparation of Yeast DNA Embedded in Agarose PlugsAnja van Brabant(adapted from Iadonato, S. P., and A. Gnirke. 1996. RARE-cleavage analysis of YACs.
PREPARATION-OF-SEQUENCING-GELS
MATERIALS:2-glass plates1 sharks -tooth comb and spacersWhatman 3 mm paper30 or 40% acrylamide-bis (19:1)10X TBEurea10% ammonium persulfateTEMED60 cc.
Preparation-of-Polyacrylamide-Gels
1. Prepare 20X TBE as:216 g Tris Base110 g Boric Acid80 mL 500 mM EDTA, pH 8.0700 mL ddH2OMix. Bring volume to 1 L. Autoclave.2. Prepare Acrylamide so
Sample-preparation-(analytical-gels)
Sample preparation and solubilization are crucial factors for the overall performance of the 2-D PAGE technique. Protein complexes and aggregates shou
EGel®-CloneWell-Agarose-Gels
实验概要Instructions are provided below for using the E-Gel®CloneWell pre-cast agarose gels with the E-Gel® iBase™ Power System. For detailed instructio
DNA电泳
DNA电泳(主要内容如下) Preparation of Agarose Gel and Electrophoresis Extraction of DNA From Agarose Gel Extraction of DNA from Acrylamide Gels DNA Marker
Preparation-of-denaturing-6%polyacrylamide-gels-for-microsatellite-analysis
Preparation of denaturing 6% polyacrylamide gels for microsatellite analysis(also for SSAP, high-resolution IRAP/ISSR and other analyses)Saadiah Jamli
DNA-Sequencing-Gels
DNA Sequencing GelsBuffers and gel solutionsLong Ranger: we started using this in early 1995. Great stuff; the best thing is that the gels are not sti
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
ELECTROPHORESIS-OF-DNA-IN-POLYACRYLAMIDE-GELS
ELECTROPHORESIS OF DNA IN POLYACRYLAMIDE GELSGel SizesSmall: 165 x 130 mmMedium: 165 x 200 mmLarge: 165 x 260 mm5% Anal
蛋白质电泳
蛋白质电泳(主要内容如下)One-Dimensional SDS-PAGETwo-Demensional SDS-PAGEProtein Electrophoresis in Agarose Gel Gel StainingRecipesOne-Dimensional SDS-PAGE·
酵母准备
Yeast DNA PreparationYeast Genomic Preparation (Gottschling Lab)Rapid method for yeast genomic DNA isolation Yeast DNA Preparation (rapid glass bead
Pulse-Field-Electrophoresis
Manipulating and analyzing DNA are fundamentals in the field of molecular biology. Indeed, separating complex mixtures of DNA into different sized fra
DNA抽提
DNA抽提(主要内容如下)· Working with DNA· DNA Extraction from Bacteria and Other Organisms· DNA Extraction from Cell and Tissue· Mitochondria DNA Isola
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
Southen杂交
Southern杂交One important thing for transfer:the weight of the object resting on top of the blotting apparatus should not exceed the weight equal to a 5
Agarose-Gel-Electrophoresis-of-DNA
1) Dissolve 1 g of agarose in 100 ml of 1X TAE or TBE buffer (gives a 1% gel). See note for making LMP agarose gel. 2) Cast the gel with the comb in p
DNA电泳(agarose胶)
DNA琼脂糖凝胶电泳 实验方法原理 利用DNA分子在琼脂糖凝胶中泳动时具有的电荷效应和分子筛效应。电荷效应是指DNA分子在高于等电点的pH溶液中带负电,在电场
DNA电泳(agarose胶)
实验材料 DNA样品试剂、试剂盒 琼脂糖 电泳缓冲液溴化乙锭 上样缓冲液仪器、耗材 电泳仪电泳漕 透射紫外灯 胶带纸 紫外成像仪
DNA电泳(agarose胶)
DNA电泳可用于:(1)分离不同大小的DNA片段;(2)鉴定目的DNA片段;(3)纯化和回收DNA片段。实验方法原理利用DNA分子在琼脂糖凝胶中泳动时具有的电荷效应和分子筛效应。电荷效应是指DNA分子在高于等电点的pH溶液中带负电,在电场中向正极移动,且相同数量的双链DNA几乎具有等量的净电荷,能以
Lambda-DNA-Preparation
Lambda DNA PreparationThis is a plate method that gives very good yield for cloning. I have combined the Promega and Maniatis protocols.Solutions T-TY
Preparation-of-Sonicated-Human-DNA
Purpose:To break up high molecular weight human placental DNA into fragment sizes of 500 bp or less which can be used as competitor DNA in Southern an
Midiprep-preparation-of-Plasmid-DNA
实验概要The PureLink™ HiPure Plasmid DNA Midiprep Kit allows purification of 100–350 μg of high-quality plasmid DNA from 15–25 mL overnight E. coli cul
Maxiprep-preparation-of-Plasmid-DNA
实验概要The PureLink™ HiPure Plasmid DNA Maxiprep Kit allows purification of 500–850 μg of high-quality plasmid DNA from 100–200 mL overnight E. coli cu
DNA凝胶电泳(DNA-agarose-gel-electrophoresis)
实验原理琼脂糖凝胶电泳是常用的用于分离、鉴定DNA、RNA分子混合物的方法,这种电泳方法以琼脂凝胶作为支持物,利用DNA分子在泳动时的电荷效应和分子筛效应,达到分离混合物的目的。DNA分子在高于其等电点的溶液中带负电,在电场中向阳极移动。在一定的电场强度下,DNA分子的迁移速度取决于分子筛效应,即分
Denaturing-Agarose-Gel-Electrophoresis-of-RNA
The overall quality of an RNA preparation may be assessed by electrophoresis on a denaturing agarose gel; this will also give some information about R