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  • EasyWaytoCloneGenesFromaPhageLibrary

    Easy Way to Clone The protocol is oriented towards a C. albicans genomic library I made in Lambda Zap II on 7/97.The overall sequence of events is: ? Titer and plate out phage ? Lift plaques onto filters and prepare them for screening ? Make a probe ? Hybridize the probe to the filters ? Wash the filters and expose to film ? Purify putative plaques ? Excise plasmid from the des......閱讀全文

    Easy-Way-to-Clone-Genes-From-a-Phage-Library

    Easy Way to Clone?The protocol is oriented towards a C. albicans genomic library I made in Lambda Zap II on 7/97.The overall sequence of events is:??

    cDNA-AMPLIFICATION-FROM-LAMBDAPHAGE-LIBRARY

    PREPARE SOLUTIONS1. SM buffer (1 L):Mix?5.8?g of NaCl,?2?g of MgSO4-7H2O,?50?mL of 1M Tris-HCl, pH 7.5,?0.5?mL of 2% gelatin, and dH2O to 1 L (Autocla

    Preparation-of-phage-particles-from-phage-vectors

    Pick up one phage vectors-containing colony with a sterile loop and put into 10 ml? 2xTY + 10 μg/l tetracycline.Shake at 200 rpm and 37 °C untill the

    Genomic-Libraries

    Genomic DNA libraries?Size of some genomes and chromosomes:Comparative Sequence Sizes(Bases)(yeast chromosome 3)350 ThousandEscherichia coli (bacteriu

    CDNA文庫

    ?CDNA文庫(主要內容如下)·?????????Construction of cDNA Library·?????????Construction of Genome DNA Library·?????????Library Screening??OthersConstruction of cD

    Screening-a-cDNA-Library

    Screening a cDNA Libraryfor use with HybriZAP zebrafish cDNA librariesObjectivecDNA library screening allows detection of expressed genes for subseque

    Phage-Titer

    IntroductionLambda phage is a commonly used vector for transgenes. Its very high rate of infectivity makes it ideal for creating large numbers of clon

    Quick-and-Easy-Isolation-of-Genomic-DNA-from-Yeast

    ProcedureTransfer 1.5 ml of liquid culture of yeast grown for 20 - 24 h at 30°C in YPD (1% yeast extract, 2% peptone, 2% dextrose) into a microcentrif

    利用人工組合轉錄因子對人類基因組掃描2

    Figure 5: Regulation of?CDH5?by TFZFs in several human cancer cell lines.Blue, cells infected with a pMX construct containing the DNA binding domain o

    Degenerate-PCR,-a-short-guide.

    What is degenerate PCR????Degenerate PCR is in most respect identical to ordinary PCR, but with one major difference. Instead of using specific PCR pr

    Degenerate-PCR

    Degenerate PCR is in most respects identical to ordinary PCR, but with one major difference. Instead of using specific PCR primers with a given sequen

    cDNA-LIBRARY-SCREENING

    PREPARE SOLUTIONS1. 10mM MgSO4, 0.2% Maltose LB (100 mL):Mix?1.0?g of Bacto-Tryptone,?1.0?g of NaCl,?0.5?g of Yeast Extract, and?1.0?mL of 1M MgSO4. A

    噬菌體的生長

    Preparing Lawn Cells for M13 Cloning?(Life Technologies)Lawn cells require the F' episome for M13 infection and may be prepared??Streaking Lambda

    DNA克隆

    DNA克隆(主要內容如下)·?????????General Procedure·?????????PCR Cloning·?????????Subcloning·?????????ET Cloning·?????????Vector Preparation·?????????Ligation Re

    The-TRC-shRNA-Design-Methods-and-Rules

    OverviewWe design shRNA molecules with an algorithm. Our algorithm uses several criteria to rank potential 21mer targets within each human and mouse R

    Construction-and-Manipulation-of-LargeInsert-Bacterial-Clone-Libraries

    Acknowledgements?The organizer of the workshop acknowledges Dr. Murray Milford, Professor and Interim Head, and Dr. Mark Hussey, Professor and Interim

    Standard-Operating-Procedures-for-T1Phage-Testing-Assay

    I. Introduction:This assay uses a lawn of phage-susceptible?E. coli?(DH10B) embedded in a layer of agarose. This top agarose lays on a bed of standard

    人工轉錄因子的部件——人類鋅指結構2

    Table 2: Binding sites and identity of ZFPs used in?VEGF?activationWe then generated artificial transcription factors by fusing the three-finger domai

    Expression-Library-Screening-(Procaryotic)-Using-APFusion-Proteins

    Outline:Bacteriophage lambda is a linear double stranded DNA, approximately 50 kB in size. The two sticky ends help the phage to recircularize after e

    The-TRC-shRNA設計方法與原則

    OverviewWe design shRNA molecules with an algorithm. Our algorithm uses several criteria to rank potential 21mer targets within each human and mouse R

    Twohybrid-analysis-of-genetic-regulatory-networks2

    2.2 Interaction mating - large scaleWith a few modifications, the procedure described above can be used to test for interactions between a single prey

    Microaspiration-of-Esophageal-Gland-Cells-and-cDNA-Library-Construction-for

    Microaspiration of Esophageal Gland Cells and cDNA Library Construction for Identifying Parasitism Genes of Plant-Parasitic NematodesIdentifying p

    M13噬菌體

    ·?????????M13 Phage?(Michael Blaber)Very useful background information about M13: its infection, replication, packing, cloning. If you are new to phag

    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

    sothing-about-Genome-walking

    Can anyone recommend a good kit for genome walking? I would like to find out the promoter sequence of a known gene. Is genome walking the way to do it

    DNA的酶學操作

    DNA的酶學操作DNA Modifying Enzymes?(Michael Blaber)Introduction to bacterial restriction/modification system. It provides very useful background knowledge

    Performing-a-hunt-by-interaction-mating

    AbstractWhen more than one bait will be used to screen a single library, significant time and resources can be saved by performing the interactor hunt

    組織學——顯微解剖

    Laser Capture Microdissection (LCM)Introduction to LCM??(BJMU)??Preparation, LCM and RNA/DNA extraction of Frozen Tissue Sections?(NIH Laser Capture M

    利用人工組合轉錄因子對人類基因組掃描

    Scanning the human genome with combinatorial transcription factor librariesPublished online: 18 February 2003, doi:10.1038/nbt794March 2003 Volume 21

    酵母人工染色體

    ·?????????Easy YAC Preparation Method?(Andrew Davies,Shaw lab)·?????????Screening YAC libraries?(Donis Keller Lab)This is a method for screening YAC l

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