毕赤酵母表达试剂盒,原始试剂盒
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引用和文献 (68)
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毕赤酵母表达试剂盒,原始试剂盒

The Original Pichia Expression Kit is designed for high-level expression of recombinant protein in the yeast Pichia pastoris. The vectors了解更多信息
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货号数量
K1710011 个试剂盒
货号 K171001
价格(CNY)
31,582.00
Each
添加至购物车
数量:
1 个试剂盒
价格(CNY)
31,582.00
Each
添加至购物车

The Original Pichia Expression Kit is designed for high-level expression of recombinant protein in the yeast Pichia pastoris. The vectors carry the HIS4 gene for selection of transformants on histidine-deficient medium. The Original Pichia Expression Kit provides all of the tools and reagents needed to express a gene of interest from the AOX1 promoter.

仅供科研使用。不可用于诊断程序。
规格
耐抗生素细菌氨苄青霉素 (AmpR)
细菌或酵母菌株GS115, KM71
克隆方法限制性内切酶/MCS
表达机制基于细胞的表达
表达系统酵母
适用于(应用)蛋白表达
产品类型表达试剂盒
蛋白标记未标记
数量1 个试剂盒
细胞类型酵母细胞
产品规格试剂盒
促进剂AOX1
种属毕赤酵母
矢量pPIC
Unit SizeEach
内容与储存
原始毕赤酵母表达试剂盒包括各 10 µg 用于细胞内表达的 pHIL-D2 和 pPIC3.5 载体以及用于分泌表达的 pHIL-S1 和 pPIC9 载体、毕赤酵母菌株 GS115 (his4)、KM71(arg4 his4 aox1::ARG4)、对照菌株 GS115 白蛋白、对照菌株 GS115 β-gal、培养基(YP 和 YNB)、原生质球转化试剂盒和各 2 µg 5´AOX1、3´AOX1 和 α-因子测序引物。在 -20°C 下储存载体和引物室温下储存菌株。妥善储存时,可保证所有组分稳定储存 6 个月。

常见问题解答 (FAQ)

当使用pPIC6/pPIC6α载体在X-33酵母株中筛选杀稻瘟菌素抗性转化株时,为什么在含300 μg/ml杀稻瘟菌素的YPD培养皿中得到的菌落有大有小?

通常,大菌落代表含pPIC6/pPIC6α整合体的转化株,而小菌落代表含pPIC6/pPIC6α非整合体的转化株。这些非整合体转化株已经转导了pPIC6/pPIC6α质粒,因此,在起始筛选过程中表现出低水平的杀稻瘟菌素抗性。在后续筛选中,这些非整合体转化株不会保持杀稻瘟菌素抗性。

当您为表达实验选择杀稻瘟菌素抗性转化株时,我们建议您从起始转化培养皿中挑选杀稻瘟菌素抗性菌落,然后在第二个含有适当浓度杀稻瘟菌素的YPD培养皿中划线。应选择可保持杀稻瘟菌素抗性的转化株用于下一步研究。

我的转化失败了。你们有何建议?

•应确保收集的是处于对数生长期的细胞(通常OD <1.0)。
•如果使用电穿孔法,应查看电穿孔仪使用手册中的推荐条件。可根据需要,改变电穿孔参数。
•使用更多的DNA。
•使用新鲜配制的感受态细胞。
•如果使用LiCl转化法,可尝试煮沸载体DNA。

我成功制备了两次Pichia的原生质球,之后就制备不成功了。培养物的OD值根本不降低。

应考虑以下几点:

1.如果所用细胞的OD值过高,则它们不能形成原生质球。不要使细胞过度生长。
2.不要使用衰老的细胞,应确保细胞处于对数生长期。
3.使用前,将酵母裂解酶混合均匀。酵母裂解酶更大程度上是一种悬液,而非溶液。
4.每次都使用新鲜配制的PEG溶液,并检查pH。

Pichia pastoris和S. cerevisiae的培养基有哪些不同种类?

以下是用于培养Pichia pastoris和S. cerevisia的营养丰富型和基本培养基:

营养丰富型培养基:

适用于S. cerevisiae和Pichia pastoris
•YPD(YEPD):酵母提取物、蛋白胨和葡聚糖
•YPDS:酵母提取物、蛋白胨、葡聚糖和山梨醇

仅适用于Pichia pastoris
•BMGY:缓冲型甘油复合培养基
•BMMY:缓冲型甲醇复合培养基

基本培养基(又名缺陷型培养基):

适用于S. cerevisiae
•SC(SD):完全合成培养基(YNB、葡聚糖(或棉籽糖或半乳糖)以及氨基酸)

适用于Pichia pastoris

•MGY:基本甘油培养基
•MD:基本葡聚糖培养基
•MM:基本甲醇培养基
•BMGH:缓冲型基本甘油培养基
•BMMH:缓冲型基本甲醇培养基

使用组成型表达载体(如pGAPZ)进行发酵,是否有推荐的实验方案?

pGAP克隆可使用以下高细胞密度实验方案。加入碳料,直至达到所需的细胞密度(细胞湿重(WCW)为300-400 克/升)。如果发酵罐中的蛋白状态良好,可增加至300–400 克/升 WCW,与甲醇诱导型克隆相似。在发酵后48小时内,可达到该密度。我们已经使用这些方案,使组成型表达载体在甘油中进行发酵,并得到良好的结果。您可能需要对发酵基础盐培养基做以下改进:

1) 在分批发酵培养基中,用2%葡聚糖代替4%甘油。
2) 在补料生长培养基中,用40%葡聚糖代替50%甘油。
3) 以12 毫升/升/小时的速度补加40%葡聚糖(Jim Cregg已经发表使用多种碳源作为底物进行表达的数据;葡聚糖带来最高表达水平)。
4) 可在培养基中加入酵母提取物和蛋白胨,维持蛋白稳定性。

警告:如果您在使用His-酵母株,使用pGAPZ转化后,酵母株依然是His-标记的。使用基本培养基发酵时,需要在发酵罐中加入组氨酸。

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引用和文献 (68)

引用和文献
Abstract
Expression and functional characterization of the mammalian intestinal peptide transporter PepT1 in the methylotropic yeast Pichia pastoris.
Authors:Doring F, Theis S, Daniel H
Journal:Biochem Biophys Res Commun
PubMed ID:9126331
The methylotrophic yeast Pichia pastoris was used for heterologous expression of the rabbit intestinal peptide transporter PepT1 and its functional characterization. PepT1 mediates the electrogenic transmembrane transport of di- and tripeptides and peptido-mimetics such as beta-lactam antibiotics and ACE-inhibitors. Functional expression of PepT1 was determined in different recombinant clones by ... More
Recombinant proteinase 3 (Wegener's antigen) expressed in Pichia pastoris is functionally active and is recognized by patient sera.
Authors:Harmsen MC, Heeringa P, van der Geld YM, Huitema MG, Klimp A, Tiran A, Kallenberg CG
Journal:Clin Exp Immunol
PubMed ID:9367410
'The open reading frame of human proteinase 3 (PR3) without the prepro- peptide was cloned and expressed in Escherichia coli (rcPR3) and in Pichia pastoris (rpPR3). The 6-histidine tagged rpPR3 was efficiently secreted into culture supernatant from which it could be purified by immobilized metal chelate chromatography. Purified rpPR3 migrated ... More
Autocatalytic processing of recombinant human procathepsin L. Contribution of both intermolecular and unimolecular events in the processing of procathepsin L in vitro.
Authors:Menard R, Carmona E, Takebe S, Dufour E, Plouffe C, Mason P, Mort JS
Journal:J Biol Chem
PubMed ID:9468501
'The autocatalytic processing of procathepsin L was investigated in vitro using purified recombinant proenzyme expressed in Pichia pastoris. Pure intermolecular processing was studied by incubating the mutant procathepsin L (C25S), which cannot autoactivate with a small amount of mature active cathepsin L. The results clearly establish that, contrary to recent ... More
Lethal effect of recombinant human Fas ligand in mice pretreated with Propionibacterium acnes.
Authors:Tanaka M, Suda T, Yatomi T, Nakamura N, Nagata S
Journal:J Immunol
PubMed ID:9036978
'Fas ligand (FasL) is a type II membrane protein. Binding of FasL to its receptor, Fas, induces apoptosis. Matrix metalloproteinase cleaves the membrane-bound human FasL to yield the active soluble form. Here, we have produced a large amount of human soluble rFasL using the yeast, Pichia pastoris. The purified rFasL ... More
Role of the cysteine residues in the alpha1,2-mannosidase involved in N- glycan biosynthesis in Saccharomyces cerevisiae. The conserved Cys340 and Cys385 residues form an essential disulfide bond.
Authors:Lipari F, Herscovics A
Journal:J Biol Chem
PubMed ID:8910350
'The Saccharomyces cerevisiae alpha1,2-mannosidase, which removes one specific mannose residue from Man9GlcNAc2 to form Man8GlcNAc2, is a member of a family of alpha1,2-mannosidases with similar amino acid sequences. The yeast alpha1,2-mannosidase contains five cysteine residues, three of which are conserved. Recombinant yeast alpha1, 2- mannosidase, produced as the soluble catalytic ... More
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