TheprotocolforLICbyExonucleaseIII
The protocol for LIC by Exonuclease III梁耀極1. Design the primers with 15-bp overlap;2. Digest the vector by proper restriction enzyme;For getting high quality vectors, there are some good advices as follows:1) The restriction sites we choose should be 5’-overhangs orblunt ends , but it shouldn’t be 3'-protruding ends ;2) Digestion by double enzymes;3) Digestion the vector overnight to make sure complete cleavage a......閱讀全文
The-protocol-for-LIC-by-Exonuclease-III
The protocol for LIC by Exonuclease III梁耀極1. Design the primers with 15-bp overlap;2. Digest the vector by proper restriction enzyme;For getting high
足跡法(Footprinting)
Footprinting Procedures·?????????DNase I Footprinting?(Mike A. Dyer)·?????????DNase I footprintingDetermining the site of binding for a protein on a D
DNA測序
DNA測序(主要內容如下)·?????????Sequencing Gel Preparation·?????????Preparation of Templates?·?????????DNA Sequencing by the Dideoxy Method·?????????DNA Sequen
關于鋰電池的化學反應式介紹
1、鋰鈷氧化物電池 在陽極處,鋰被氧化。鋰離子與電子一起從碳中釋放出來: LiC6→xLi++xe?+C6LiC6→xLi++xe?+C6 在陰極處,鋰離子被二氧化鋰吸收,電極被還原,因為它也從電路接收電子: Li1?xCoO2+xLi++xe?→LiCoO2Li1?xCoO2+xLi+
ELISPOT-Protocol
實驗概要The ?Elispot (Enzyme Linked Immuno-Spot) assay provides an effective method ?of measuring the antibody or cytokine production of immune cells on t
Immunoblot-Protocol
This method was successful in our lab using prostate tissue and for our specific objectives. Investigators must be aware that they will need to tailor
ELISPOT-protocol
實驗概要The procedure ?below is a general guideline procedure for ELISPOT. Abcam ELISPOT kits ?have been designed for detection of various cytokines and g
PCR-protocol
PCR reactionProtocol for 50μl reaction - adjust amounts if necessary, for a 20μl reaction use the same volumes of primer and dNTP-mix, but adjust the
RLGS-protocol
A. Preparation of DNA SolutionIn the case of rice, for example This method may be appllicable for many grass species and some other plants.????????
ELISA-protocol
ELISA protocol:1.取5-10ul BMMY表達上清用0.05M NaHCO3稀釋到100ul鋪ELISA板,37度或室溫振蕩大于1小時。注意一定要做一個GS115空菌株表達上清作為陰性對照,最好還找一個帶有histag的蛋白作為陽性對照。2.TPBS洗板3次,方法:倒掉鋪板液,倒置于
NAi-protocol
siRNA protocolsOur current strategy with siRNA is to synthesis relatively small amounts enzymatically and use these to test for efficiency by western
RNAi-protocol
?siRNA protocolsOur current strategy with siRNA is to synthesis relatively small amounts enzymatically and use these to test for efficiency by western
ELISPOT-Protocol
實驗概要The ?Elispot (Enzyme Linked Immuno-Spot) assay provides an effective method ?of measuring the antibody or cytokine production of immune cells on t
Immunoprecipitation-Protocol
實驗概要Immunoprecipitation ?is a procedure by which proteins or peptides that react specifically ?with an antibody are removed from solution and examined
RNA-FISH-on-cultured-cells-in-interphase
IntroductionFluorescence?in situ?hybridization (FISH) has become a widely used method in genome and molecular genetic studies. The technique is highly
DNA的誘變和甲基化
·?????????In Vitro Mutagenesis Using Altered Sites?(Bowtell Lab)?In vitro Mutagenesis with dut ung single stranded DNA?(Hahn Lab)·?????????Site-direct
Bacteria-Culture-Protocol
Bacteria Culture ProtocolBy 徐曉政1、TBS Medium Preparation:Prepare 1L of TBS medium contains:Tryptone 12gYeast extract 24gNaCl 5gSodium Succinate 5gGlyce
Intracellular-Staining-Protocol
1.?Fix cells- Add16% formaldehyde directly into culture medium to obtain a final concentration of 1.5% formaldehyde.2. Incubate in fixative for 10 min
Tissue-Harvest-Protocol
TISSUES TO BE PROCURED(minimally and preferably within 5-8 hours after death):1. Brain2. Liver3. Muscle4. Skin5: Others as the specific case dictatesP
Silver-Staining-Protocol
1x 40min - overnight?????50% MeOH, 12% Acetic Acid1x 30min??????????????????????????????????50% MeOH, 12% Acetic Acid, 0.05% 37% Formaldehyde3x 20min?
Migration-Assay-Protocol
Materials to be prepared beforehand:1) FBS free medium2) 10% FBS medium3) Cell migration filter insert ( Transwell?, 12mm Diameter, 12 μm Pore Size.)P
Protocol-of-Northern-blot
Protocol of Northern blot質粒的轉化和擴增質粒的鑒定目的基因片段的切割3.1樣品雙酶切(175μl水解體系)DW 115μlBuffer B(10×) 17.5μlBaM H 15μlPst I 17μlDNA(MMP-9) 16μlBSA 4.5μl37℃水浴,3h。3.2
Protocol-for-Trichl...
實驗概要The ?efficiency of nucleotide incorporation in DNA/RNA polymerization ?reactions (e.g. transcription, reverse transcription, and DNA ?replication)
Western-Blot-Protocol
一、提取抗原蛋白將提取RNA途中留存的樣品,加入150μl 100%酒精充分混勻,靜置5min(RT), 2000×g , 4℃離心5min,?吸取上清至新管中,?加入750μl異丙醇,?混勻,?靜置10min(RT), 12000×g, 4℃離心10min,?棄上清,?加入1ml 0.3mol/L
Sandwich-ELISA-Protocol
實驗概要The ?Sandwich ELISA measures the amount of antigen between two layers of ?antibodies (i.e. capture and detection antibody). The antigen to be ?mea
RNA-Isolation-Protocol
Stabilize RNAStart with 15 ml E. coli Culture containing 7.5* 109 cells (OD600= 0.2 Dilute cells or scale up)Pipet 30 ml of RNAProtect Bacteria Reagen
Dot-Blot-Protocol
a. Label nitrocellulose membrane (using a pencil) to identify protein elution fractions.b . Pipette 2μl from each fraction onto the membrane, allow th
Urea-Lysis-Protocol
Urea?lysis?buffer????????????9M Urea, 2.5mM EDTA, 2.5mM EGTA, 1% DTE, 4% CHAPS????????????make 10ml and aliquot 10x1ml, freeze at -70°C?Lysate?prepara
cDNA/AFLP-Protocol
Preparation of Para-magnetic beads from Promega cat#Z5482:a) suspend magnetic particles in bottle - transfer 200 ul (200 ug) of beads per sampleof RNA
RNA-Isolation-Protocol
RNA Isolation Protocol(Revised 5-15-2003)Stabilize RNAStart with 15 ml E. coli Culture containing 7.5* 109?cells (OD600= 0.2 Dilute cells or scale up)