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TAIL-PCR to clone flanking sequence from Feldmann's lines (Chun-Ming Liu)
• Autoradiography (William H. Heidcamp)
  This procedure involves the incorporation of a radioactive substance into a cell, and subsequent detection of that material through the use of a photographic emulsion. The primary source used for cell biology is an organic molecule containing tritium, the radioactive form of hydrogen. Radioactive carbon, phosphorous and iodine are occasionally utilized, but tritium has inherently more resolution than any of the others
• KDO Assay (Hancock Lab) (Viewed by IE only)
• Lambda-Tnphoa Mutagenesis of Cloned Genes in E Coli (Hancock Lab) (Viewed by IE only)
• Liposome Preparation (Hancock Lab) (Viewed by IE only)
• Liposome Swelling Assay (Hancock Lab) (Viewed by IE only)
• LPS Isolation (Hancock Lab) (Viewed by IE only)
• Disruption by Fusion PCR (David Amberg and Ellen Beasley)
  1) In separate PCR reactions, amplify the 5' and 3' ends of the gene of interest with primers about 200 bases apart. Primer 2 should begin with 24 nts complementary to the m13 forward primer(GTC GTG ACT GGG AAA ACC CTG GCG) and primer 3 should begin wit h 24 nts complementary to the m13 reverse primer (TCC TGT GTG AAA TTG TTA TCC GCT). PCR amplify the marker using the m13 forward and reverse primers. 
• Actin Capture Assay
• In-Gel Digest Protocol (Siuzdak Lab)
  Procedure for the Micropreparation of Internal Protein Fragments for Amino Acid Sequencing
• Codon Usage Table
• Chromatin IP (CHIP assay)
• Yeast Cell Micromanipulation
  Protocol for making support rod with fiber optic needle attached
• Methionine Labeling (Hancock Lab) (Viewed by IE only)
• Methylation of Fatty Acides (Hancock Lab) (Viewed by IE only)
• MIC Determination Microtitre Broth Dilution  (Hancock Lab) (Viewed by IE only)
• Muramic Acid Assay (Hancock Lab) (Viewed by IE only)
• Nituocefin Assay for Outer Membrane Permeability  (Hancock Lab) (Viewed by IE only)
• NPN Uptake Assay (Hancock Lab) (Viewed by IE only)
• Osmotic Shock Procedures (Hancock Lab) (Viewed by IE only)
• Oxidase Test (Hancock Lab) (Viewed by IE only)
• PBP Assay (Hancock Lab) (Viewed by IE only)
• Petri Plate Grid (Hancock Lab) (Viewed by IE only)
• Phage Progagation (Hancock Lab) (Viewed by IE only)
• Phenol Sulphuric Acid Assay (Hancock Lab) (Viewed by IE only)
• Phosphate Assay (Hancock Lab) (Viewed by IE only)
• Phosholipid Extraction (Hancock Lab) (Viewed by IE only)
• Porin F Purification (Hancock Lab) (Viewed by IE only)
• Preparation of Lipid A (Hancock Lab) (Viewed by IE only)
• Protein and LPS Stains (Hancock Lab) (Viewed by IE only)
• Protease Digestion of Outer Membranes  (Hancock Lab) (Viewed by IE only)
• Protocol for Thermal Mouse Model (Hancock Lab) (Viewed by IE only)
• Separation of Outer and Inner Membranes  (Hancock Lab) (Viewed by IE only)
• Synthesis of Dansyl-polymyxin (Hancock Lab) (Viewed by IE only)
• Transformation of Helicobacter Pylori (Hancock Lab) (Viewed by IE only)
• Transposon Mutagenesis (Hancock Lab) (Viewed by IE only)
• Triparental Mating (1)  (Hancock Lab) (Viewed by IE only)
• Triparental Mating (2) (Hancock Lab) (Viewed by IE only)
• TSBD Trypticase Soy Broth Dialysate (Hancock Lab) (Viewed by IE only)
• Whole Cell Crosslinking (Hancock Lab) (Viewed by IE only)
• Whole Cell Phosphate Uptake Assay  (Hancock Lab) (Viewed by IE only)
• Whole Cell Protein and LPS Gels (Hancock Lab) (Viewed by IE only)
• X-gal & AP Staining Protocol (Cepko Lab)

Plant related

Crosses (Schneitz Lab)
• Pest Control (Schneitz Lab)

Lipid Protocols

• Phosphate Assay (Jiandi Zhang)
• DEAE Column (SJ)
• DEAE column: FPLC (SJ)
• Desalting Acidic Glycosphingolipids (SJ)
• Arachidonic Acid Labeling (SJ)
• AA & Metabolite Quantitation of Cell Pellets Post-AA Labeling (SJ)
• AA & Metabolite Quantitation of Media Post-AA Labeling (SJ)
• Neutralizing Arachidonic Acid (SJ)
• Preparation of bOG-DOPG Mixed Micelles (SJ)
• [3H] Choline Labeling and TNF Treatment of HL-60 Cells (SJ)
• DGK Assay (SJ)
• DGK Membrane Preparation (SJ)
• Column Purification of Demethylated Sphingomyelin (SJ)
• Purification of Demethylated Sphingomyelin (SJ)
• Drying Lipids with Liquid Nitrogen Evaporator (SJ)
• Glycosphingolipid analysis (SJ)
• In vitro Sphingomyelinase Assay (SJ)
• Labelled Sphingmyelin Synthesis (SJ)
• After Using the Nitrogen Evaporator (SJ)
• Phosphate Assay by Suprya Jayadev (SJ)
• Purification of Demethylated Sphingomyelin (SJ)
• Sphingomyelin Quantitation Post-choline Labeling of HL60 Cells (SJ)
• Sphingomyelin Mass Measurement (SJ)
• Thin Layer Chromatography (SJ)
• Micro-Glutathione Assay (P. J. Hansen Lab)

Animal Techniques

• Transplants of Adult Tissue into Fat Pads (Mammary Gland Biology,NIH)
• Transplants of Embryonic Tissue into Fat Pads (Mammary Gland Biology,NIH)
• Renal Capsule Grafting (Mammary Gland Biology,NIH)
• Milking a Mouse (Mammary Gland Biology,NIH)

Drosophila Related Protocols

• Drosophila Head Collection
• Drosophila DNA Prep
• Drosophila RNA Prep
• Immunohistochemistry on Drosophila Brains

C. Elegans Protocols

• C. elegans gene knockout protocol
• cleaning worm strains
• culturing worms
• dye filling sensory neurons
• EMS mutagenesis
• F2 mutant screen
• freezing worms
• integrating arrays
• lethal phase determination
• liquid culture of worms
• making males
• microinjection
• egg laying in response to food
• timing/staging development
• worm genomic Southerns
• worm RNA prep
• Ammonium Sulfate Binding (Devreotes Lab)

Biochemistry

Quantitation of Epitope-tagged GPCR's by Biotin Labeling(Von Zastrow lab)
This protocol is specifically designed for measuring the agonist-induced degradation of FLAG and HA-tagged GPCRs expressed on the plasma membrane of Human Embryonic Kidney (HEK) 293 cells.

Flow Cytometry Assay to measure Internalization of GPCR's (Von Zastrow lab)
Internalization of receptor is measured as the reduction of receptors on the plasma membrane surface. Surface receptors are labeled with fluoresent antibodies which is in turn measured using a flow cytometer. The antibodies recognize an epitope engineered onto the N-terminus of the GPCR.

Methylation Analysis

• Bisulfite Treatment of DNA (Issa Lab)
• Methylation-Sensitive PCR (MSP) (Issa Lab)
• Bisulfite-PCR (for restriction and/or sequencing) (Issa Lab)
• Southern Blot Analysis (Issa Lab)
• Methylated CpG Island Amplification (MCA) (Issa Lab)
• DNA-Methyltransferase Assay (Issa Lab)
• Bisulfite Mutagenesis (Technical Tips Online) (To view this page, you need registration. it's free)
  This protocol is  used to analyze the methylation profile of  CpG dinucleotides of DNA. 

Xenopus Egg Extractology

• Crude Extract Prep for In Vitro Spindle Assembly. (Mitchison Lab)
  High Speed Supe Extract Prep
    
• Crude Extract Immunodepletion (Mitchison Lab)
    
• HSS Extract Immunodepletion (Mitchison Lab)

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