预存质粒
PET31b,PET41bPGEM 7ZF
PGEX-2T
pProEX-HTa
pProEX-HTb
pProEX-HTc.
基因酷,您好!我是基因酷linsea1124,我已认真阅读《资源保证协议》,并同意签署。
质粒:PET31b(+)
我预共享的质粒基本信息:
载体名称:PET31b(+)
载体抗性:amp
载体大小:5742bp
载体宿主:E. coli
载体特点:The pET-31b(+) vector is designed for cloning and high-level expression of peptide sequences fused with the 125aa ketosteroid isomerase protein (1). The unique [i]Alw[/i]N I cloning site allows the unidirectional insertion of of tandemly repeated peptide coding regions separated by methionine codons. Note that the sequence is numbered by the pBR322 convention, so the T7 expression region is reversed on the vector map
网站链接:[url=http://www.emdbiosciences.com/html/NVG/pETTable.html]http://www.emdbiosciences.com/html/NVG/pETTable.html[/url]
质粒:pET 41b(+)
载体名称:pET 41b(+)
载体抗性:Kan
载体大小:5932bp
载体宿主:E.coli
载体特点:The pET-41 series is designed for cloning and high-level expression of peptide sequences fused with the 220 aa GST•Tag™ protein. Note that the sequence is numbered by the pBR322 convention, so the T7 expression region is reversed on the vector map ([url=http://www.emdbiosciences.com/docs/docs/PROT/TB239.pdf][color=#0000ff]TB239[/color][/url]). The f1 origin is oriented so that infection with helper phage will produce virions containing single stranded DNA that corresponds to the coding strand. Vector encoded sequence can be completely removed when cloning into the [i]Psh[/i]AI site and then cleaving the GST fusion protein with Enterokinase...
网站链接: [url=http://www.emdbiosciences.com/product/70557]http://www.emdbiosciences.com/product/70557[/url]
图谱及序列信息可在网站链接中查询.
载体名称:pGEM 7ZF(+)
载体抗性:Amp
载体大小:2997bp
载体宿主:Ecoli
载体特征:The pGEM®-7Zf(+) and pGEM®-7Zf(–) Vectors are derivatives of the pGEM®-3Zf(+) Vector and contain the origin of replication of the filamentous phage f1. These plasmids serve as standard cloning vectors, as templates for in vitro transcription and can be used for the production of circular ssDNA. These plasmids contain SP6 and T7 RNA polymerase promoters flanking a region of multiple cloning sites within the α-peptide coding region of β-galactosidase (1). Insertional inactivation of the α-peptide allows recombinant clones to be identified directly by color screening on indicator plates when using appropriate [i]E. coli[/i] strains (e.g., JM109). The multiple cloning region is unique and includes restriction sites for ApaI, AatII, SphI, XbaI, XhoI, EcoRI, KpnI, SmaI, Csp45I, ClaI, HindIII, BamHI, SacI, BstXI and NsiI. This arrangement is designed specifically for generating unidirectional deletions with the Erase-a-Base® System. pGEM®-7Zf(+) and pGEM®-7Zf(–) Vectors are identical except for the orientation of the f1 origin.
网站链接: [url=http://www.promega.com/catalog/catalogproducts.aspx?categoryname=productleaf_215&ckt=1]http://www.promega.com/catalog/catalogproducts.aspx?categoryname=productleaf_215&ckt=1[/url]
载体名称:PGEX-2T
载体大小:4948bp
载体抗性:Amp
载体特性:原核GST融合表达载体
网站链接:[url]http://www4.gelifesciences.com/aptrix/upp01077.nsf/Content/Products?OpenDocument&[/url];parentid=976038&moduleid=38859&zone=Proteomics
载体名称:pProEX-HTa,pProEX-HTb,pProEX-HTc
载体大小:4751bp,4779bp,4780bp
载体抗性:Amp
载体特征:见Invitrogen公司网站链接
网站链接: [url=https://tools.invitrogen.com/search/index.cfm?searchterm=pproex-hta&fuseaction=search.simplesearch&navFilter=category:Vector%20Maps]https://tools.invitrogen.com/search/index.cfm?searchterm=pproex-hta&fuseaction=search.simplesearch&navFilter=category:Vector%20Maps[/url]
[[i] 本帖最后由 linsea1124 于 08-10-24 13:33 编辑 [/i]] linsea1124酷友,您好!您预共享的资源对于基因酷是“新颖的”,请您将以下信息站内短消息给我们:
一、个人信息包含内容如下:
您的真实姓名:
学习或工作单位:
联系电话(包括手机):
QQ或MSN:
E-mail:
目前研究项目简介:(最少50字,主要说明项目的研究目的、难点和取得的结果。)
邮寄地址和邮编:
以上信息主要是为了更加及时的给您邮寄资源,以及对共享资源的有效跟踪。基因酷对您的私人信息绝对保密,敬请酷友放心!(站内短信发给我们)
二、资源基本信息包含内容如下:
您对该资源的使用经历,主要包含该资源在您的实验室的使用频率;您的实验室最后一次使用该资源的日期,使用该资源的结果如何;如果可以希望您也能说明一下您使用该资源做过什么实验;
您获取该资源的途径;
对该资源您做过哪方面的验证工作,比如测序,表达,检测等;
以上信息主要是为了配合保藏中心的鉴定工作。基因酷保证对这些信息的绝对保密,敬请您放心。 您好,请教pProEX-HTa,pProEX-HTb,pProEX-HTc是哪个系列的质粒,方便我们归类到资源列表。谢谢! 非常感谢斑竹帮忙把图谱帖出来!
pProEX-HT a,pProEX-HTb,pProEX-HTc是Invitrogen公司的原核融合表达载体,带六聚组氨酸标签. 资源已经于10月12日寄出,麻烦管理员注意查收一下
回复 5# 同窗酷友 的帖子
17号时,还没收到您发出的资源,正常来讲,那么多天了,应该到了才是。您用单号查下它到哪了吧 您好,今天已收到资源,原来您是用挂号信寄过来的,建议以后用快递。时间久了,担心资源出问题了。还有,您寄来的资源是6个,没有PGEM 7ZF。怎么帖子上的PGEX-2T的信息不见了的?麻烦您再次补上,谢谢 不好意思,主要是发快递不太方便,所以用了挂号信,没想到要这么久PGEM-7ZF可能是临时遗漏了,下次补上 管理员,你好!不知道我寄过去的质粒通过鉴定没有? 您好!昨天刚好做完鉴定,5个资源通过了鉴定,PGEX-2T转了几次都没长。 好的,那我最近把PGEX-2T连同PGEM-7ZF再寄过去 好的,感谢您对基因酷的支持!
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