FlagHAdoubletagIP
實驗概要Isolate the unknown protein that could interact with bait from cell lysate, for potential Mass spectrometry.主要試劑50mM Tris, pH8.020 mM glycerol b-phosphate, pH 7.520 mM NaF0.5 mM sodium Orthovannadate5 mM sodium pyrophosphate 137mM NaCl1mM EDTA1% Triton X10010% glycerol實驗步驟 Havest the cells by centrifugation at 1,000 rpm for 3 min. Wash the cells with ice cold PBS twice.Resuspend the cell pellet with 5 v......閱讀全文
Antibody-Purification-using-Protein-A,-Protein-G,-or-Protein-L-Agarose
實驗概要This protocol is designed as a quick purification method for antibodies from mammalian sera, ascites, and cell culture supernatants. It should
Antibody-Purification-using-Protein-A,-Protein-G,-or-Protein-L-Agarose
實驗概要This ?protocol is designed as a quick purification method for antibodies from ?mammalian sera, ascites, and cell culture supernatants主要試劑?Protein
Radioiodination-of-protein
Radioiodination (by Jun Takagi,6/16/2000)Purpose and backgroundsPrinciple of radioiodinationAddition of oxidizing reagents (such as chloramine-T or pe
Protein-Electrophoresis
DefinitionAmino acids, nucleotides, polypeptides, and other compounds in a colloidal state can be separated by the application of external voltages wh
Protein-Crystallization
Background:Proteins, like many molecules, can be prompted to form crystals when placed in the appropriate conditions. In order to crystallize a protei
The-Determination-of-Proteinprotein-Interactions-by-the-Matingbased-...
Dynamic and reversible protein–protein interactions have a pivotal function in all living cells. For instance, protein–protein interactions are in
Eukaryotic-protein-translation
The scanning translation initiation model suggests that 40S ribosomal subunit preloaded with factors bind to the 5’ end of the mRNA near the cap. The
LOWRY-PROTEIN-ASSAY
The Lowry procedure is one of the most venerable and widely-used protein assays, being first described in 1951 [Lowry et al.,?J. Biol. Chem. 193: 265-
Protein-Kinase-A-at-the-Centrosome
Protein kinase A regulatory subunit RIIalpha (PKA-RIIa) is tightly bound to centrosomal structures during interphase through interaction with the A-ki
Bradford-protein-assay
Bradford protein assayConsiderations for useThe Bradford assay is very fast and uses about the same amount of protein as the Lowry assay. It is fairly
BIURET-PROTEIN-ASSAY
BIURET PROTEIN ASSAYMATERIALSBiuret ReagentBovine serum albumin (BSA)Spectrophotometer and tubesPROCEDUREPrepare standard dilutions of BSA containing
Bradford-–-Protein-Determination
Bradford – Protein DeterminationIntroductionA rapid and accurate method for the estimation of protein concentration. The technique is simpler, faster
Protein-A-Purification-of-Antibody
1. Reagents(1) Affi-gel Protein-A Agarose (BioRad #153-6153)(2) MAPS II Binding Buffer (BioRad # 153-6161)(3) 0.314 g/ml diH2O(4) MAPS II Elution Buff
Protein-Staining-Procedures
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
Protein-Assay-(Spectrophotometer)
Protein Assay (Spectrophotometer)Use BSA (bovine serum albumin) 1mg/ml stock solution (1ml Eppendorf tubes) for standard curve.Place 0, 2, 5, 10, 15,
Lowry-–-Protein-Determination
Lowry – Protein Determination(From Protein Protocols on CD-ROM Humana Press, 1998 - Section 1-2 The Lowry Method for Protein Quantitation Jakob H. Wat
Acetone-precipitation-of-protein
This procedure is suitable for recovering proteins from most aqueous solvents and from SDS containing buffers. It is not recommended for proteins diss
Preparing-a-Selenomethionyl-Protein
PurposeThe protocol describes how to prepare selenomethionyl (Se-Met) protein using a regular E.coli strain. Selenium can be used for phase determinat
Protein-arginine-methylation
Typical modification sites: RGG box or RXR sequence motifs R-arginine, G-glycine,X-any aminoacid.Enzymes catalysing protein arginine methylation: PRMT
Protein-purification;-actin
Protein purification; actin ? ? ?Overview?? ACTINThe most abundant muscle and non-muscle cytoskeletal protein. MW 42 kDa, 374/375 amino acids; various
Basic-Protein-Chemistry-Techniques
Coomassie Blue Stain:? (for gels)?1) Combine 225 ml Methanol with 225 ml ddH2O.?2) Add 0.5 grams of Coomassie Blue.?3) Just before use, add 50 ml acet
Biorad-Protein-Assay:-Bradford
Biorad Protein Assay: BradfordStandards: 1 mg/ml BSA stock- dilute 1:10 to get 0.1 mg/ml BSAAdd To get H-2O20 μl 2 μg/ml 780 μl40 μl 4 μg/ml 760 μl60
Cyanogen-Bromide-digestion-of-protein
1. Proteins are TCA precipitated and washed with acetone, then dried.2. The CNBr should be brought to room temperature in the hood and used ONLY in th
Coupling-Antibodies-to-Protein-A-or-G
1. use 2 mg of antibody per ml wet beads (use appropriate antibody/protein A or G combination).2. mix antibodies with beads and bind at room temperatu
Protein-G-Purification-of-Antibodies
1. Reagent and Materials(1) Hi-Trap Protein G Column (Pharmacia Biotech #17-0404-01)(2) 20 mM Sodium Phosphate Buffer, pH 7.01.084 g NaH2PO4, anhydrou
Angiotensin-Protein-Kinase-Assay
James Hardwick's angiotensin assay protocolThis specific procedure was developed to assay the activity of the Lck kinase expressed from a retrovir
Basic-Protein-Chemistry-Techniques
實驗概要Basic Protein Chemistry Techniques實驗步驟Coomassie Blue Stain:? (for gels)?1) Combine 225 ml Methanol with 225 ml ddH2O.?2) Add 0.5 grams of Coomassi
Mechanism-of-Protein-Import-into-the-Nucleus
Nuclear pore complexes (NPCs) are large proteinaceous assemblies that provide the only known portals for exchanging macromolecules between the nucleus
In-Vitro-Protein-Ubiquitination-Assay
Ubiquitination is one of the most important posttranslational modifications in all eukaryote organisms. Ubiquitin-activating enzyme (E1), ubiquiti
Western-Blot-with-Platelet-Protein
OUTLINEWestern blot is a wide used technique to identify a target protein/s for the certain antibody.PROTOCOLPrepare platelets.Lyse washed platelets (