&

生物資源

當(dāng)前位置：首頁 - 生物資源 - 生物資源

產(chǎn)品名稱：pMal-c4X

貨號	規(guī)格	價格	訂購數(shù)量	是否現(xiàn)貨
ZK1576	1μg(20μl,50ng/μl)	870	- +	有貨

產(chǎn)品介紹

■ 基本信息

別名:	pMalc4X
啟動子:	Tac
復(fù)制子:	pBR322
終止子:	rrnB T1 terminator
質(zhì)粒分類:	大腸桿菌載體；pMal系列表達質(zhì)粒
質(zhì)粒大小:	6645bp
質(zhì)粒標(biāo)簽:	N-MBP, N-Factor Xa
原核抗性:	Amp
克隆菌株:	DH5a
培養(yǎng)條件:	37度
表達宿主:	BL21(DE3)
培養(yǎng)條件:	37℃，有氧，LB
誘導(dǎo)方式:	IPTG或乳糖及其類似物
5'測序引物:	MalE引物: 5-GGTCGTCAGACTGTCGATGAAGCC-3;MBP-F: 5-gatgaagccctgaaagacgcgcag-3
3'測序引物:	pBad-5 5-gatttaatctgtatcagg-3; M13-F: 5-TGTAAAACGACGGCCAGT-3

■ 質(zhì)粒屬性

質(zhì)粒宿主:	大腸桿菌
質(zhì)粒用途:	蛋白表達
片段類型:	ORF
片段物種:	空載體
原核抗性:	Amp
真核抗性:
熒光標(biāo)記:

■ 質(zhì)粒簡介

The pMAL?-4 vectors (Figure 1) provide a method for expressing and purifying a protein produced from a cloned gene or open reading frame. The cloned gene is inserted downstream from the malE gene of E. coli, which encodes maltose-binding protein (MBP), resulting in the expression of an MBP fusion protein (1,2). The MBP in these vectors has been engineered for tighter binding to amylose. The method uses the strong “tac” promoter and the malE translation initiation signals to give high-level expression of the cloned sequences (3,4), and a one-step purification of the fusion protein using MBP’s affinity for maltose (5). The vectors express the malE gene (with or without its signal sequence) fused to the lacZα gene. Restriction sites between malE and lacZα are available for inserting the coding sequence of interest. Insertion inactivates the β-galactosidase α-fragment activity of the malE-lacZα fusion, which results in a blue to white color change on Xgal plates when the construction is transformed into an α-complementing host such as TB1, JM107 or NEB 5-alpha Competent E. coli (6,7). When present, the signal peptide on pre-MBP directs fusion proteins to the periplasm. For fusion proteins that can be successfully exported, this allows folding and disulfide bond formation to take place in the periplasm of E. coli, as well as allowing purification of the protein from the periplasm (8). The vectors carry the lacIq gene, which codes for the Lac repressor. This keeps expression from Ptac low in the absence of IPTG induction. The pMAL-4 vectors also contain the sequence coding for the recognition site of a specific protease, located just 5′ to the polylinker insertion sites. This allows MBP to be cleaved from the protein of interest after purification. The pMAL-c4X and pMAL-p4X vectors that are included in the system encode the site for Factor Xa (9, 10). Factor Xa cleaves after its four amino acid recognition sequence, so that few or no vector-derived residues are attached to the protein of interest, depending on the site used for cloning. pMAL vectors containing sites for alternative proteases are also available (Figure 1). The vectors pMAL-c4G and pMAL-p4G encode the site for Genenase?I , which cleaves following the sequence His-Tyr. The vectors pMAL-c4E and pMAL-p4E encode the site for Enterokinase , which cleaves following the sequence Asp-Asp-Asp-Asp-Lys.

■ 質(zhì)粒圖譜

■ 質(zhì)粒序列

質(zhì)粒序列請下載：ZK1576 pMal-c4X大腸表達質(zhì)粒.txt

用戶姓名：	*
用戶手機：	*
電子郵箱：
單位名稱：	*
留言內(nèi)容：	*
驗證碼：	看不清，換一張 *