AntibodyPurificationusingProteinA,ProteinG,orProteinLAgarose
实验概要This protocol is designed as a quick purification method for antibodies from mammalian sera, ascites, and cell culture supernatants. It should be noted that if the starting material is serum or ascites the final preparation will contain endogenous host IgG as well as specific antibodies. In general, the presence of this endogenous IgG should not interfere with assays using the antibodies. The immunogl......阅读全文
Antibody-Purification-using-Protein-A,-Protein-G,-or-Protein-L-Agarose
实验概要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
实验概要This protocol is designed as a quick purification method for antibodies from mammalian sera, ascites, and cell culture supernatants主要试剂 Protein
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-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
Purification-of-Antiserum-or-Ascites-by-Protein-A/G-Chromatography
1、Required Materials and Equipment(1) Protein A or G agarose gel column (10 ml or 5 ml of packed beads; see guidelines below for choice of protein A o
Protein-purification;-actin
Protein purification; actin Overview ACTINThe most abundant muscle and non-muscle cytoskeletal protein. MW 42 kDa, 374/375 amino acids; various
Protein-Expression-and-Purification-Protocol
Step 1: Transform appropriate DNA plasmid into BL21(DE3) E. coli cells. These cells must be competent. (Protocol for how to make competent cells.)a) T
troponin蛋白纯化-Protein-purification:-troponins
Overview TROPONINS The calcium-dependent regulatory protein complex located on the thin actin filaments of muscle comprises of TnC (17.8 kDa), TnI (2
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
Purification-of-Kar3-Motor-Domain-Protein
Purification of Kar3 Motor Domain ProteinMaterialsInduced cells (2 - 5 g pellet of pET/Kar3 in BL31(DE3)pLysS host cells) (See note #1)HEM buffer =10
Studying-Arabidopsis-Envelope-Protein-Localization-and-Topology-Using-...
Chloroplasts are metabolically important organelles that perform many essential functions within plant cells. The chloroplasts can be subdivided i
Protein-L树脂填料应用说明
Protein L也是一种免疫球蛋白结合蛋白,来源于从消化链球菌马格努斯。不同于Protein A和Protein G,Protein L结合的是抗体分子的轻链。由于没有重链的参与,比起Protein A和Protein G,Protein L可以结合更多种类型的抗体。Protein L可以
抗体纯化
Antibody PurificatioinPurification of IgG Using Protein A- or Protein G-Agarose (KPL) Purifying Antibodies (Perkin-Elmer)Precipitation MethodsProtein
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
单克隆抗体
· Tips and hints for the storage of antibodies (Synaptic Systems)· Purification of IgG Using Protein A- or Protein G-Agarose(KPL)·
Jacobs:Protocol-Total-Protein-Isolation-Using-RIPA-Lysis-Buffer
MaterialsRIPA buffer (RIPA buffer enables the extraction of cytoplasmic, membrane and nuclear proteins and is compatible with many applications, inclu
Signaling-Pathway-from-GProtein-Families
G-aS-coupled receptors stimulate adenylyl cyclase (AC), which synthesizes cAMP from ATP. In contrast Gai-coupled receptors inhibit AC and so reduce cA
GProtein-Signaling-Through-Tubby-Proteins
The tubby gene product is expressed in the brain and has been implicated by mouse genetics in obesity and other disorders such as blindness. Structura
Activation-of-PKC-through-G-protein-coupled-receptor
G-protein coupled receptors (GPCRs) transduce a variety of signals from the extracellular environment across the plasma membrane. One of the common si
Protein-A--G亲和层析的原理
对于IgG的纯化,大部分情况下我们都会选择使用Protein A或Protein G进行亲和层析。因为它们对于IgG的Fc段具有特异性的亲和作用,而对于其他杂蛋白没有或者只有很弱的结合。通常,仅仅凭借Protein A或Protein G一步亲和层析就可使蛋白纯度达到≥90%。
蛋白质纯化(protein-purification)实用技术2
7.密度多数蛋白质的密度在1.3~1.4g/cm3之间,分级分离蛋白质时一般不常用此性质,不过对含有大量磷酸盐或脂质的蛋白质与一般蛋白质在密度上明显不同,可用密度梯度法离心与大部分蛋白质分离。8.基因工程构建的纯化标记通过改变cDNA在被表达的蛋白的氨基端或羧基端加入少许几个额外氨基酸,这个加入的标
蛋白质纯化(protein-purification)实用技术3
10.非极性基团之间作用力溶质分子中的非极性基团与非极性固定相间的相互作用力(非选择性分散力或伦敦力)大小与溶质分子极性基团与流动力相中极性分子在相反方向上相互作用力的差异进行分离。因其流动相中的置换剂是极性小于水的有机溶剂(如甲醇、乙腈、四氢呋喃等),这些有机溶剂可能使许多蛋白质分子产生不可逆的变
蛋白质纯化(protein-purification)实用技术1
研究的最后还是要看基因表达产物,无论是用于检测还是用于棉衣保护,都需要将表达出的蛋白质分离和纯化,然而蛋白质性质各异,故纯化方法不同,现共享一些基本的纯化方法,以飨读者:蛋白质的一级、二级、三级和四级结构决定了它的物理、化学、生物化学、物理化学和生物学性质,综述了不同蛋白质之间的性质存在差异或者改变
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