Acris ABCA0060694说明书

 

Acris ABCA0060694说明书

Human IgM (Fc5 mu specific) (AP)

 

名称:

人IgM(Fc5 mu特异性)(AP)

产品组:

一抗

产品编号:

ABCA0060694

价钱:

€330.00

指示价格:

N / A

 

 

 

 

数量:

1

单克隆/多克隆:

多克隆

 

 

同型对照(Y / N):

没有

纯化(Y / N):

没有

装载控制:

没有

描述:

人免疫球蛋白M.

笔记:

制造商:Acris Antibodies GmbH

 

 

 

 

 

 

应用

 

共轭类型:

酶检测

 

主办:

兔子

 

 

 

 

产品信息

 

限制:

仅供研究和体外使用。不用于诊断或治疗工作。

 

R1341AP Human IgM (Fc5 mu specific) antibody

Search for all “Human IgM”

人IgM的产品描述

性质:(Fc5 mu特异性)
介绍:AP

人IgM的特性

产品分类

二抗

目标类别

  • 人IgM抗体

数量

1毫克

同义词

人免疫球蛋白M.

介绍

美联社

克隆

多克隆

主办

兔子

运到

*

数据表提取

免疫原

免疫原:

人IgM(Fc5μ)片段

应用

适用于免疫印迹(Western印迹或斑点印迹),ELISA和免疫组织化学以及其他基于磷酸酶 – 抗体的酶测定,需要批次间的一致性。
推荐稀释度:在标准捕获ELISA中使用pNPP对硝基苯基磷酸酯作为底物在室温下测定该产物对1.0μg人IgG。建议对该产品使用1:500至1:2,000的重构浓度的工作稀释液。

浓度

1.0 mg / ml(通过280 nm的紫外吸光度)

一般读物

共轭:从Avarameas和Ternyrock修改,免疫化学32; 1175年1971年。

存储

将抗体(未稀释)保存在2-8°C。
不要冻结!
冷冻碱性磷酸酶缀合物将导致
酶活性的显着损失。
仅在立即使用前稀释。
保质期:发货一年。

格式

标签:

碱性磷酸酶(小牛肠)(分子量140,000道尔顿)
AP

纯化:

免疫亲和层析

缓冲系统:

0.05M三氯化锆,0.15M氯化钠,0.001M氯化镁,0.0001M氯化锌,50%(v / v)甘油; pH 8.0,含10mg / ml牛血清白蛋白(BSA,IgG和无蛋白酶)作为稳定剂和0.01%(w / v)sodium azide作为防腐剂。

州:

液体(无菌过滤)纯化的IgG级分。

特异性

特异性:

通过免疫亲和层析从单特异性抗血清制备该产物,使用与琼脂糖珠偶联的人IgM,然后进行固相吸附以除去任何不需要的反应性。
通过免疫电泳测定导致针对抗碱性磷酸酶(小牛肠),抗兔血清,人IgM和人血清的单一沉淀弧。
通过ELISA确认特异性,与其他人重链或轻链同种型的交叉反应性低于1%。

 

 

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1:强大的进口辐射能力,血清、抗体、耗材、大部分限制进口品等。

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Phosphosolutions公司Anti-ABCA4 (Rim Protein)产品代理


Phosphosolutions公司Anti-ABCA4 (Rim Protein)产品代理

简要描述:公司概况

背景
基因工程– Phosphosolutions是*代可以完整描绘人体的遗传物质序列的企业。
蛋白质体学项目:Phosphosolutions是第二代试图将所有体内蛋白质表达出来的企业。
PhosphoSolutions公司—第三步我们将超越蛋白质体学 进而 专注于磷蛋白质。

our focus 专业特色
PhosphoSolutions公司专注于蛋白质组学中的一个(10-20

详细介绍

产品咨询

 Antibodies 抗体

特异性磷抗体:Detection and quantitation of changes in the state of phosphorylation of specific proteins is of great utility in the quest to establish the function of a given protein and the consequences of its reversible phosphorylation. Two methods commonly used to measure protein phosphorylation and dephosphorylation in cell preparations employ prelabeling with 32Pi or back phosphorylation. These methods continue to be very effective and have advantages for many test systems, but they do have several practical and theoretical limitations (Nestler and Greengard, 1984). Based in large part on the successful use of short synthetic peptides to produce epitope-targeted antibodies (Lerner, 1982;Sutcliffe et al., 1983), an immunochemical approach became an attractive alternative for detecting changes in the state of phosphorylation of specific proteins at a specific site. The use of phosphorylation state-specific antibodies takes advantage of the sensitivity and selectivity afforded by immunochemical methodology, combined with relatively simple preparation and potentially broad applications.

The first report of phosphorylation-dependent antibodies appeared in 1981, when polyclonal antibodies that could detect phosphotyrosine-containing proteins were produced by immunization with benzyl phosphonate conjugated to keyhole limpet hemocyanin (KLH) (Ross et al., 1981). Shortly thereafter, Nairn and colleagues reported the production of serum antibodies that distinguished between the phospho- and dephospho-forms of G-substrate, a protein localized to cerebellar Purkinje cells and phosphorylated by cGMP-dependent protein kinase (Nairn et al., 1982). A synthetic heptapeptide, Arg-Lys-Asp-Thr-Pro-Ala-Leu, corresponding to a repeated sequence surrounding two phosphorylated threonyl residues in the intact protein, served as antigen. Rabbit antisera against a peptide-KLH conjugate were specific for the dephospho-form of G-substrate. Phospho-specific antibodies were prepared by immunization of rabbits with the purified phosphoprotein, phosphorylated in vitro to a stoichiometry of 2 mol/mol with cGMP-dependent protein kinase. Despite this initial success, other attempts in our laboratory to produce phospho-specific polyclonal antisera by immunization with the phospho-form of intact proteins were not very successful, probably because of two significant factors. First, many phosphorylated proteins are believed to undergo rapid dephosphorylation during immunization, regardless of the route of injection, leading to the loss of the desired phospho-epitope. Second, holoproteins generally contain multiple immunogenic epitopes; this decreases the probability that colonal dominance for a phospho-specific epitope will be obtained.

Taking a more direct approach utilizing phosphorylated and unphosphorylated forms of synthetic phosphopeptides, we developed a general protocol for the production of phosphorylation state-specific antibodies for substrates with established site(s) of phosphorylation (Czernik et al., 1991)). In early stages of our development of this methodology, phosphopeptides were routinely prepared by enzymatic phosphorylation (Czernik et al., 1991). Although this approach remains perfectly valid today, the preparation of synthetic phosphopeptides using Fmoc derivatives of phosphoamino acids has become the state-of-the-art (Czernik et al., 1995;Czernik et al., 1996). Likewise, we have examined the use of both polyclonal and monoclonal techniques for antibody production. Given the high success rate that we and others have obtained with the polyclonal technique, it has become the method of choice, because it is an easier and less costly method for the average laboratory. However, when appropriate, this approach can be readily adapted for monoclonal antibody production.

参考文献

1. Czernik AJ, Girault J-A, Nairn AC, Chen J, Snyder G, Kebabian J, Greengard P (1991) Production of phosphorylation state-specific antibodies. Methods Enzymol 201: 264-283.

2. Czernik AJ, Mathers J, Mische SM (1997) Phosphorylation state-specific antibodies. Neuromethods: Regulatory Protein Modification: Techniques & Protocols 30: 219-250.

3. Czernik AJ, Mathers J, Tsou K, Greengard P, Mische SM (1995) Phosphorylation state-specific antibodies: preparation and applications. Neuroprotocols 6: 56-61.

4. Lerner, R. A. Tapping the immunological repertoire to produce antibodies of predetermined specificity. Nature 299, 593-596. 1982.

5. Nairn AC, Detre JA, Casnellie JE, Greengard P (1982) Serum antibodies that distinguish between the phospho- and dephospho-forms of a phosphoprotein. Nature (Lond ) 299: 734-736.

6. Nestler, E. J. and Greengard, P. Protein Phosphorylation in the Nervous System. Nestler and Greengard. Protein Phosphorylation in the Nervous System. [8], 255-299. 1984. New York, Wiley. 

8. Sutcliffe JG, Shinnick TM, Green N, Lerner RA (1983) Antibodies that react with predetermined sites on proteins. Science 219: 660-666.

主营产品清单如下:

Item: Anti-ABCA4 (Rim Protein)
Category:  
Sub-Category:  
SKU/Catalog Number: 115-ABCA4
Datasheet:  click to view

 

SKU Price Formulation Applications Amount Qty
115-ABCA4 $325.00 Affinity purified, monoclonal antibody WB, IHC 100 µl

 

virogen 246-A说明书

virogen 246-A说明书

 

ANTI-HCV NS4B IGG2B MAB

CATALOG #246-A

概要

抗HCV NS4B IgG2b(单克隆)针对重组抗原产生。

抗丙型肝炎NS4B单克隆抗体
产品目录号:246-A
产品描述:针对重组抗原产生的HCV NS4B IgG2b(单克隆)
特异性:HCV NS4B抗原
表位aa 1710-1730
克隆:2-H1
来源:小鼠
纯度:蛋白G纯化的
缓冲液/组成:1 X PBS pH 7.2;0.01%叠氮化纳
浓度:1 mg / ml,可根据要求提供大量
储存:长期:-80°C
短期:4°C (三个月或更短)
应用:ELISA〜10-6 
Western blot,(1: 1000)
IHC(低温恒温器肝脏切片-1 
: 20)运输:冷敷

该产品仅用于实验室研究或进一步制造,不应用于人体治疗或诊断应用。

 

 

 

antibodychain ABCA0060904说明书

antibodychain为您的研究提供更多帮助!antibodychain将整个抗体产业聚集在一个平台开辟了*的网络,市场营销和销售机会。antibodychain平台为顾客提供几万种抗体及相关研究产品。包括抗体,裂解,蛋白质,肽等。antibodychain致力为客户提供更的产品与服务。

antibodychain ABCA0060904说明书

大鼠IgG(H + L链)(生物素)

名称: 大鼠IgG(H + L链)(生物素)
产品组: 二抗
产品编号: ABCA0060904
价钱: €220.00 指示价格: N / A
数量: 2
单克隆/多克隆: 多克隆
纯化(Y / N): 没有

 

描述:

 

大鼠免疫球蛋白G.

 
   
应用
共轭类型: 荧光检测
共轭: 生物素
主办: 兔子
   
产品信息
限制:

仅供研究和体外使用。不用于诊断或治疗工作。

   

 

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phosphosolutions 115-ABCA4 说明书

世界*实验材料供应商phosphosolutions上海金畔生物为其中国代理,phosphosolutions在一直是行业的*,一直为广大科研客户提供zui为的产品和服务,上海金畔生物一直秉承为中国科研客户带来的产品,的服务, phosphosolutions就是为了给广大科研客户带来更加完善的产品和服务,您的满意将是我们zui大的收获

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我们公司zui大优势是强大的采购,

1:基本什么都能进口,血清,抗体,耗材,还有部分限制进口的,

2 货品全,现经营过700多个品牌,基本所有生物试剂耗材都可以进口,特别是冷偏的产品那就更有优势,

3:提供加急服务,一般1-2周到货,超过时限加急费全免

4:价格公道,绝大部分价格有优势,当然不能保证100%产品都是,因为意味着没有服务.

5:良好的信誉,大部分客户我们提供货到付款服务,客户包括清华,北大 交大 复旦,中山等100多所大学,ROCHE,阿斯利康,国药 fisher500多家公司

6:我们还是santa,Advanced Biotechnologies Inc;Athens Research & Technology, bangs, BBInternational, crystalchem, dianova, FD Neurotechnologies, Inc. FormuMax Scientific, Inc; Genebridege; Glycotope Biotechnology GmbH; iduron; Innovative Research of America Ludger  neuroprobe; omicronbio; Polysciences; prospecbi; QA-BIOquickzymeRESEARCH DIETS, INCsterlitechsysyTriLink BioTechnologies, Incworthington-biochem;zyagen;……几十家国外公司代理

7:我们还从事invitrogenqiagen; abcam ;sigma;neb; roche;merck; rnd; BD; GE; pierce; BioLegend….等*批发