Coimmunoprecipitationassays
co-IP assays can be performed between endogenous proteins or transiently or stably expressed exogenous - usually tagged - proteins. The advantage to using endogenous proteins is the avoidance of protein overexpression and tagging that can lead to artifacts. The advantage to using exogenously expressed tagged proteins is the generally high specificity of the anti-tag antibody and the ease with which a negative control......阅读全文
Agglutination-Assays
Agglutination AssaysREFERENCE: Lanyi, B., and T. Bergan. Methods in Microbiology, Vol 10: 93-168. BACTERIAL AGGLUTINATION: Bacterial agglutination is
Cellulase-assays
实验概要 Cellulase enzymes show activity during the ripening of some fruits, where their effects on cell walls results in softening of the frui
Carbohydrate-Assays
Carbohydrate AssaysREFERENCE: Wright and Rebers, Anal. Biochem. 49: 307-319, 1972.OBJECTIVE: To determine the relative amounts ofLPS carbohydrates pre
Cellulase-assays
Cellulase enzymes show activity during the ripening of some fruits, where their effects on cell walls results in softening of the fruit. In cases of p
Matrigel-invasion-assays
OverviewMatirgel is considered as basement membrane and generated from EHS sarcoma. Matrigel contains not only basement membrane components (collagens
Microtubule-Binding-Assays
MaterialsSiliconized ultracentrifuge microfuge tubesGTP-depleted microtubules6X SDS loading dye1X SDS loading dyeCoomassie Brilliant Blue R 250 (0.8%
Cytotoxicity-Assays-Protocol
Cytotoxicity Assays ProtocolCell-mediated cytotoxicity was determined by using a standard microcytotoxicity assay. Briefly, target cells were pelleted
DNA-Fragmentation-Assays-for-Apoptosis
Protocol I: Triton X-100 Lysis BufferIn 96 flat-wells plate, incubate 4x10 6 target cells (40 wells of 105 per well) with desired concentration of eff
PLAQUE-ASSAYS-FOR-ADENOVIRUS-TITRATION
-Set up 60 mm dishes of P11 cells to be 100 confluent at time of infection. -Remove medium from dishes, add 0.2 to 0.5 ml virus and adsorb for 30 – 60
cAMP分析-cAMP-Assays
cAMP AssaysGouzel Karimova and Daniel LadantUnite Postulante de Biochimie des Interactions Macromoleculaires, Departement de Biologie Structurale et C
SAPK/Jun-kinase-assays
Preparation of cell lysate:1. For cells in suspension, grow in DMEM with 10% FCS and then the day before you do the experiment spin the cells down (1
Coimmunoprecipitation-assays
co-IP assays can be performed between endogenous proteins or transiently or stably expressed exogenous - usually tagged - proteins. The advantage to u
Microtubule-(MT)/Organelle-Motility-Assays
Rapidly thaw and immediately place on ice one aliquot each of axonemes, Golgi or ER membranes, 45 uM tubulin, rat liver cytosol, and 20x energy regene
Nuclear-RunOn-Transcription-Assays
Nuclear “run-on” (or “run-off”) transcription assays have been used to obtain quantitative information about the relative rates of transcription o
Fragment-Complementation-and-Coimmunoprecipitation-Assays-for-...
Plant disease resistance (R) proteins confer protection against specific pathogens or pathogen isolates. R proteins function by recognizing pathog
Preparation-of-Luciferin-for-In-Vitro-and-In-Vivo-Bioluminescent-Assays
Preparation of Luciferin forIn Vitro Bioluminescent AssaysMaterials• D-Luciferin Firefly, potassium salt, 1.0 g /vial(Caliper Life Sciences Part Numbe
Preparation-of-Luciferin-for-In-Vitro-and-In-Vivo-Bioluminescent-Assays
实验概要Reagent for immunoassay, ligand binding assay and ligand receptor assay in which luciferin is covalently bonded to a molecule having biological
ATPase-Assays-with-32PATP
MaterialsPurified Motor Protein, 20-80 µMNucleotide Mix =50 mM Mg·ATP gamma-32P-ATP to give 5 000 - 10 000 cpm/nmol 10 mM HEPES, pH 7.2 1 mM EGTA 1 mM
Preparation-of-Luciferin-for-In-Vitro-and-In-Vivo-Bioluminescent-Assays
实验概要Reagent for immunoassay, ligand binding assay and ligand receptor assay in which luciferin is covalently bonded to a molecule having biological
Steady-State-ATPase-Assays-Coupled-Enzyme-System
MaterialsTubulin (>5 mg/mL)100 mM Mg·GTP4 mM Taxol in DMSOPM =100 mM PIPES pH 6.82 mM EGTA1 mM Mg2SO4Motor protein (>95% purity; 15-20 µM)Cuvettes (20
Flow-Cell-Assays-with-Microtubules:-Motility/Dynamics-in-Fluorescence
Flow cell assays are very useful for studying microtubule motility, microtubule dynamics, kinetochore-microtubule interactions and action of severing/
In-Vitro-prostate-colony-and-sphereforming-assays
1. Prostates were dissected, minced into small pieces with a steel blade, and digested with 0.8 mg/ml collagenase in 10 ml of primary cell medium/
实验室自动化与筛选协会2013亚洲会展短期培训课程简介
短期培训课程I :生物制剂研发中的高通量筛选 Junma Zhou,博士,上海药明康德新药开发有限公司 刘洁颖博士,上海药明康德新药开发有限公司 In Scope of Short Course - Overview of high-throughput techniques in
体外荧光法检测核内体早期动力学
A fluorescence-based in vitro assay for investigating early endosome dynamicsSina V Barysch1,2, Reinhard Jahn1 & Silvio O Rizzoli2ABSTRACTEarly endoso
Guide-to-Cell-Proliferation-and-Apoptosis-Methods
Chapter 1: Cell Death - Apoptosis and Necrosis1.1Introduction21.1.1Terminology of cell death21.1.2Differences between necrosis and apoptosis31.1.3Apop
Chloroplast-Phenomics:-Systematic-Phenotypic-Screening-of-Chloroplast-...
Chloroplast Phenomics: Systematic Phenotypic Screening of Chloroplast Protein Mutants in ArabidopsisAs part of a project to analyze chloroplast functi
siRNAs结合生物芯片的实验设计1
Ambion and Applied Biosystems have joined forces to provide a complete convenient, solution for performing gene silencing experiments and validating t
高通量筛选的FLIPR荧光检测法介绍
近年来,光学测定技术在美、英两国研究人员在高通量筛选检测中,努力进行了光学测定方法的研究,建立了大量的非同位素标记测定法,如用分光光度检测法筛选蛋白酪氨酸激酶抑制剂、组织纤溶酶原激活剂等,均获得成功。 放射性检测技术美国学者GanieSM在高通量药物筛选研究中,应用放射性测定法,特别是亲和闪烁
siRNAs结合生物芯片的实验设计2
Figure 2. Silencer ™ siRNA Validation Data Generated Using Applied Biosystems TaqMan® Gene Expression Assays. The indicated Silencer Validated siRNAs
Phosphatidylinositol-4Kinase-and-Phosphatidylinositol-4Phosphate-5K...
Phosphatidylinositol 4-Kinase and Phosphatidylinositol 4-Phosphate 5-Kinase AssaysInositol lipid kinases are perhaps the easiest and most straightforw