pIZ/V5-His 载体试剂盒
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Invitrogen™

pIZ/V5-His 载体试剂盒

The InsectSelect™ Kit features the pIZ/V5-His vector for high-level expression in a variety of insect cells. This exceptionally small vector了解更多信息
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货号数量
V800001
又称 V8000-01
1 kit
货号 V800001
又称 V8000-01
价格(CNY)
13,692.00
1 kit
添加至购物车
数量:
1 kit
价格(CNY)
13,692.00
1 kit
添加至购物车
The InsectSelect™ Kit features the pIZ/V5-His vector for high-level expression in a variety of insect cells. This exceptionally small vector has several features that facilitate expression, analysis, and detection of recombinant protein in insect cells:

• The OpIE2 promoter for constitutive expression
• The Zeocin™ resistance gene for rapid selection of stably transfected cell lines
• C-terminal V5 epitope and polyhistidine (6xHis) sequence for detection with Invitrogen's Anti-V5 Antibody and rapid purification using nickel-chelating resin
仅供科研使用。不可用于诊断程序。
规格
产品类型昆虫细胞表达载体
蛋白标记位置(至您的基因)C-端
数量1 kit
载体pIZ
克隆方法限制性内切酶/MCS
产品线InsectSelect™
促进剂OplE2
蛋白标记His 标签 (6x)、V5 抗原决定簇标签, V5 Epitope Tag
Unit Size1 kit
内容与储存
InsectSelect™ 试剂盒包括各 20 µg 超螺旋冻干 pIZ/V5-His 和 pIZ/V5-His/CAT、2 µg 冻干 OpIE2 反向测序引物、1 g Zeocin™、Cellfectin™ 试剂和 1 L 用于选择的昆虫细胞系的培养基。Sf9 细胞随附 GIBCO™ Grace 昆虫培养基,High Five™ 细胞随附 GIBCO™ Express Five™ 无血清培养基。pIZ/V5-His 载体试剂盒仅包含上述表达载体和引物。将冷冻的昆虫细胞储存于液氮。将培养基和 Cellfectin™ 试剂储存于 +4°C 下。将所有其他试剂储存于 -20°C 下。正确存放时,所有试剂均可保证 6 个月的稳定。

常见问题解答 (FAQ)

在昆虫细胞中表达重组蛋白,是否有必要加入Kozak序列?

尽管Kozak序列在哺乳细胞翻译起始中的重要性已被证明,但昆虫细胞中是否也严格遵循Kozak规则仍有争议。确定其重要性的唯一方法是,对相同蛋白从不同起始序列的表达进行直接对比。即使这样,一种蛋白实现最佳表达所使用的规则可能并不适合其它蛋白。以下四篇文献证明了Kozak序列对昆虫细胞中的表达效率无任何影响:

•Hills D, Crane-Robinson C (1995) Baculovirus expression of human basic fibroblast growth factor from a synthetic gene: role of the Kozak consensus and comparison with bacterial expression. Biochim Biophys Acta 1260(1):14–20.
•Ranjan A, Hasnain SE (1995) Influence of codon usage and translational initiation codon context in the AcNPV-based expression system: computer analysis using homologous and heterologous genes. Virus Genes 9(2):149–153.

我需要在克隆目的基因时在其中包含一个核糖体结合位点(RBS)或Kozak序列吗?

ATG通常对于高效的翻译启始是足够的,尽管翻译效率要视目的基因而定。最佳的建议应是保持cDNA中天然起始位点,除非确定这一位点的功能性不理想。如果从表达的角度来考虑,推荐构建并测试两种载体,一个具有天然的起始位点,另一个具有保守的Kozak序列。通常情况下,所有N-端融合型表达载体都已包含了一个RBS或翻译起始位点。

Shine-Dalgarno和Kozak序列有何区别?

原核生物mRNA含有Shine-Dalgarno序列,也称为核糖体结合位点(RBS),它是由AUG起始密码子5’端的多嘌呤序列AGGAGG组成。该序列与16S rRNA 3’端的互补,有助于mRNA有效结合到核糖体上。同理,真核生物(特别是哺乳动物)mRNA也含有完成有效翻译所需的重要序列信息。然而,Kozak序列不是真正的核糖体结合位点,而是一种翻译起始增强子。Kozak共有序列是ACCAUGG,其中AUG是起始密码子。-3位的嘌呤(A/G)具有重要作用;若-3位是一个嘧啶(C/T),翻译过程会对-1、-2和+4位的改变更敏感。当-3位从嘌呤变为嘧啶时,可使表达水平降低多达95%。+4位对表达水平的影响相对较小,可以使表达水平降低约50%。

注:果蝇的最佳Kozak序列稍有不同,酵母完全不遵循这些规则。见下列参考文献:
•Foreign Gene Expression in Yeast: a Review. Yeast, vol. 8, p. 423-488 (1992).
•Caveneer, Nucleic Acids Research, vol. 15, no. 4, p. 1353-1361 (1987).

Do I need to include a Kozak sequence for expression of recombinant proteins in insect cells?

While the importance of a Kozak consensus sequence in translation initiation has been demonstrated in mammalian cells, there seems to be some debate as to whether the Kozak rules are as stringent in insect cells. The only way to determine its importance would be a direct comparison of expression of the same protein from different initiation sequences. Even then, the rules for optimal expression of one protein may not hold for another. Here are two references which indicate that a Kozak consensus sequence does not have any effect on efficiency of expression in insect cells:

- Hills D, Crane-Robinson C (1995) Baculovirus expression of human basic fibroblast growth factor from a synthetic gene: role of the Kozak consensus and comparison with bacterial expression.
- Biochim Biophys Acta 1260(1):14-20.
- Ranjan A, Hasnain SE (1995) Influence of codon usage and translational initiation codon context in the AcNPV-based expression system: computer analysis using homologous and heterologous genes. Virus Genes 9(2):149-153.

Do I need to include a ribosomal binding site (RBS/Shine Dalgarno sequence) or Kozak sequence when I clone my gene of interest?

ATG is often sufficient for efficient translation initiation although it depends upon the gene of interest. The best advice is to keep the native start site found in the cDNA unless one knows that it is not functionally ideal. If concerned about expression, it is advisable to test two constructs, one with the native start site and the other with a Shine Dalgarno sequence/RBS or consensus Kozak sequence (ACCAUGG), as the case may be. In general, all expression vectors that have an N-terminal fusion will already have a RBS or initiation site for translation.

Find additional tips, troubleshooting help, and resources within our Protein Expression Support Center.

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