EasySelect™ Pichia Expression Kit
본 제품은 LMO 제품으로, 고객 분께서 LMO 신고 시스템을 통해 직접 수입 신고를 진행해주셔야 합니다. 자세히보기
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인용 및 참조 문헌 (10)
Invitrogen™

EasySelect™ Pichia Expression Kit

EasySelect™ Pichia Expression Kit는 yeast Pichia pastoris에서 단백질 생산에 필요한 모든 성분을 제공합니다. EasySelect™ Kit에는 Pichia 세포 transformation을 할자세히 알아보기
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제품 가격(KRW)
2,817,000
Online offer
Ends: 31-Dec-2025
3,313,000
할인액 496,000 (15%)
Each
카트에 추가하기
EasySelect™ Pichia Expression Kit는 yeast Pichia pastoris에서 단백질 생산에 필요한 모든 성분을 제공합니다. EasySelect™ Kit에는 Pichia 세포 transformation을 할 수 있는 Pichia yeast strain, expression vector, reagent가 들어있습니다. Zeocin™ antibiotic로 high-copy number transformed variant를 쉽게 스크리닝할 수 있습니다.

Pichia pastoris expression system의 장점:
Pichia 세포를 E. coli처럼 쉽게 배양합니다.
• 다른 미생물 발현 세포보다 높은 세포 밀도를 얻을 수 있습니다.
• 다른 미생물 발현 시스템보다 세포 당 많은 단백질을 생성합니다.
• 진핵 생물 단백질 처리, 단백질 접힘(protein folding), post-translational modification의 장점이 있습니다.
• 진탕 플라스크(shake flask)에서 산업 규모 발효까지 쉽게 확장할 수 있습니다.

입증된 단백질 발현 시스템
Pichia pastoris는 30년 이상 전세계 실험실 및 업계에서 인간을 비롯한 여러 종에서 수 백가지 단백질 생성에 사용되고 있습니다(Ref 1, 2, 3).Pichia pastoris는 박테리아(E. coli) 또는 효모(Saccharomyces cerevisiae)처럼 쉽게 성장할 수 있으면서도 이런 시스템에서 많은 장점을 제공합니다(Ref 4).Pichia pastoris는 박테리아나 다른 효모보다 높은 세포 밀도로 성장할 수 있습니다.Pichia pastoris는 메탄올을 탄소원으로 성장할 수 있어 상대적으로 저렴하게 산업 수준으로 확장할 수 있습니다.

AOX1 Promoter의 힘
EasySelect™ Pichia Expression Kit는 Pichia alcohol oxidase 1 (AOX1) 유전자에서 promoter를 사용해 단백질 생성을 촉진합니다. Pichia pastoris는 유일한 탄소원으로 메탄올에서 성장할 수 있습니다. 단일 메탄올을 탄소원으로 성장 시, AOX1 mRNA는 최대 5%의 total mRNA를 나타내고 AOX1 효소가 세포 무게의 최대 30%가 될 수 있습니다(Ref 5).

EasySelect™ Pichia Expression system은 pPICZ 및 pPICZα vector와 함께 제공됩니다.pPICZ 및 pPICZα vector에는 multiple cloning site (MCS)가 들어있어 AOX1 promoter의 통제 하에 원하는 유전자를 삽입할 수 있습니다. pPICZ 및 pPICZα vector에는 c-Myc tag도 들어있어 쉽게 검출할 수 있고 polyhistidine (6xHis) tag가 들어있어 단백질을 쉽게 검출하고 정제할 수 있습니다.

Pichia pastoris는 자연적으로 몇 개의 단백질을 분비하기 때문에 pPICZα vector에서 세포 외 신호 서열을 이용해 배양 배지로 단백질 분비를 촉진하여 downstream 정제를 간편하게 할 수 있습니다.

Zeocin™ Antibiotic으로 high-copy number 가능
EasySelect™ Pichia Expression Kit는 Zeocin™ antibiotic을 이용해 형질 전환된 Pichia 세포를 선택합니다. pPICZ 및 pPICZα vector에는 Zeocin™ antibiotic의 내성을 발하는 Streptoalloteichus hindustanus (Sh ble)의 bleomycin 유전자가 들어있습니다. pPICZ 및 pPICZα vector는 Pichia genome에 안정적으로 삽입될 수 있습니다. Zeocin™ antibiotic 농도를 높여 통합수와 단백질 발현 수준이 높은 클론을 쉽게 선정할 수 있습니다.

EasySelect™ Pichia Expression Kit에는 다음 구성품이 들어있습니다.
• 배양 시작을 위한 Pichia pastorisE. coli strain의 stab vial.
• 형질 전환을 위한 competent Pichia cell 제조 시약.
• 관심 유전자를 삽입할 수 있는 AOX1 promoter 기반의 pPICZ 및 pPICZα vector.
• pPICZ vector에 유전자 삽입을 보장하는 sequencing primer.
• 형질 전환된 Pichia cell 선정을 위한 Zeocin™ antibiotic.

연구용으로만 사용할 수 있습니다. 진단 절차에 사용할 수 없습니다.

관련 링크
pPICZ A, B, C vector용 산물 삽입 보기 (PDF).
pPICZα A, B, C vector용 산물 삽입 보기(PDF).
Zeocin™ antibiotic용 산물 삽입 보기(PDF).
Invitrogen에서 이용할 수 있는 Pichia 프로토콜 제1판에서 Pichia pastoris 사용에 대해 더 알아보기.
Invitrogen의 다른 Pichia 발현 시스템에 대해 알아보기.

참고문헌

1. Cereghino JL, Cregg JM.Heterologous protein expression in the methylotrophic yeast Pichia pastoris.FEMS Microbiol Rev. 2000 Jan;24(1):45-66. [PubMed]
2. Cereghino GP, Cereghino JL, Ilgen C, Cregg JM.Production of recombinant proteins in fermenter cultures of the yeast Pichia pastoris.Curr Opin Biotechnol. 2002 Aug;13(4):329-32. [PubMed]
3. Cregg JM. Introduction: distinctions between Pichia pastoris and other expression systems. Methods Mol Biol. 2007;389:1-10. [PubMed]
4. Cregg JM, Tolstorukov I, Kusari A, Sunga J, Madden K, Chappell T. Expression in the yeast Pichia pastoris. Methods Enzymol. 2009;463:169-89. [PubMed]
5. Cregg JM, Madden KR, Barringer KJ, Thill GP, Stillman CA. Functional characterization of the two alcohol oxidase genes from the yeast Pichia pastoris. Mol Cell Biol. 1989 Mar;9(3):1316-23. [PubMed]
For Research Use Only. Not for use in diagnostic procedures.
사양
항생제 내성 박테리아Zeocin™ (ZeoR)
박테리아 또는 효모 균주GS115, KM71H, X-33
클로닝 방법Restriction Enzyme⁄ MCS
발현 메커니즘Cell-Based Expression
발현 시스템Yeast
용도(애플리케이션)Protein Expression
제품라인EasySelect
제품 유형Expression Kit
단백질 태그His Tag (6X), c-Myc Epitope Tag
수량1 Kit
선택 제제(진핵)Zeocin
셀 유형Yeast Cells
형식Kit
프로모터AOX1
P. pastoris
VectorpPIC
Unit SizeEach
구성 및 보관
The EasySelect Pichia Expression Kit includes 20 μg each of the plasmids pPICZ A, B, and C and pPICZα A, B, and C; Pichia pastoris strains X-33 (wild-type), GS115 (his4), KM71H (arg4 aox1::ARG4), and control strains for both intracellular and secreted expression; 250 mg Zeocin™ antibiotic; media (YP and YNB), EasyComp™ Pichia Transformation Kit, 2 μg each 5' AOX1, 3' AOX1, and α-factor sequencing primers. The pPICZ and pPICZα vectors are also available separately. A lacZ positive expression control is provided with pPICZ.

Store strains at +4°C. Store vectors and primers at -20°C. All components are guaranteed stable for 6 months when properly stored.

자주 묻는 질문(FAQ)

When selecting for blasticidin-resistant transformants in the X-33 strain using pPIC6/pPIC6α vectors, why do I get large and small colonies on YPD plates containing 300 µg/ml blasticidin?

Generally, large colonies represent transformants containing pPIC6/pPIC6α integrants, while small colonies represent transformants containing pPIC6/pPIC6α non-integrants. These non-integrants have transduced the pPIC6/pPIC6α plasmid, and therefore, exhibit a low level of blasticidin resistance in the initial selection process. Upon subsequent screening, these non-integrant transformants do not retain blasticidin resistance.

When choosing a blasticidin-resistant transformant for your expression studies, we recommend that you pick blasticidin-resistant colonies from the initial transformation plate and streak them on a second YPD plate containing the appropriate concentration of blasticidin. Select transformants that remain blasticidin-resistant for further studies.

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

My transformation is not working. Do you have any suggestions?

Here are some suggestinos:

- Make sure that you have harvested cells during log-phase growth (OD <1.0 generally).
- If electroporation is being used, see the electroporator manual for suggested conditions. Vary electroporation parameters if necessary.
- Use more DNA.
- Use freshly made competent cells.
- If the LiCl transformation method is being used, try boiling the carrier DNA.

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

My spheroplasting of Pichia worked twice, but hasn't worked since. The OD of the culture simply does not drop.

Here are some things to consider:

- If the OD of cells that are used is too high, they will not spheroplast. Do not overgrow cells.
- Do not use old cells and make sure that they are in log phase of growth.
- Make sure to mix zymolyase well before using. Zymolyase is more of a suspension than a solution.
- Make the PEG solution fresh each time and check the pH.

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

What are the different kinds of media used for culturing Pichia pastoris and S. cerevisiae?

Following are the rich and minimal media used for culturing Pichia pastoris and S. cerevisiae:

Rich Media:
S. cerevisiae and Pichia pastoris
YPD (YEPD): yeast extract, peptone, and dextrose
YPDS: yeast extract, peptone, dextrose, and sorbitol

Pichia pastoris only
BMGY: buffered glycerol-complex medium
BMMY: buffered methanol-complex medium

Minimal Media (also known as drop-out media):
S. cerevisiae
SC (SD): Synthetic complete (YNB, dextrose (or raffinose or galactose), and amino acids)

Pichia pastoris
MGY: minimal glycerol medium
MD: minimal dextrose
MM: minimal methanol
BMGH: buffered minimal glycerol
BMMH: buffered minimal methanol

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

Is there a recommended protocol for fermentation using constitutive expression vectors such as pGAPZ?

Use the following high cell density protocol for pGAP clones. Feed carbon until the desired density is reached (300 to 400 g/L wet cell weight (WCW)). If the protein is well-behaved in the fermenter, increase to 300-400 g/L WCW as with methanol inducible clones. These densities can be reached in less than 48 hours of fermentation. We have fermented constitutive expressers on glycerol using these protocols with good results. Some modifications to the Fermentation Basal Salts Medium that you might want to make are:

1) Substitute 2% dextrose for the 4% glycerol in the batch medium.
2) Substitute 40% dextrose for the 50% glycerol in the fed-batch medium.
3) Feed the 40% dextrose at 12 mL/L/hr (Jim Cregg has published data on expression using several carbon sources as substrates; dextrose gave the highest levels of expression).
4) Yeast extract and peptone may be added to the medium for protein stability.

One warning: If you are working with His- strains, they remain His- after transformation with pGAPZ. Fermentation in minimal medium will require addition of histidine to the fermenter.

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

View all EasySelect™ Pichia Expression Kit FAQs

인용 및 참조 문헌 (10)

인용 및 참조 문헌
Abstract
Fas ligand deficiency in HIV disease.
Authors:Sieg S, Smith D, Yildirim Z, Kaplan D
Journal:Proc Natl Acad Sci U S A
PubMed ID:9159165
'Apoptosis is postulated to be involved as an anti-viral immune mechanism by killing infected cells before viral replication has occurred. The Fas-Fas ligand interaction is a powerful regulator of T cell apoptosis and could potentially act as a potent anti-viral immune mechanism against T cell tropic virus such as human ... More
A composite Ets/Pit-1 binding site in the prolactin gene can mediate transcriptional responses to multiple signal transduction pathways.
Authors:Howard PW, Maurer RA
Journal:J Biol Chem
PubMed ID:7673116
'Binding sites for the tissue-specific transcription factor, Pit-1, are required for basal and hormonally induced prolactin gene transcription. Although Pit-1 is phosphorylated in response to several signaling pathways, the mechanism by which Pit-1 contributes to hormonal induction of gene transcription has not been defined. Recent reports suggest that phosphorylation of ... More
Expression and secretion of a biologically active glycoprotein hormone, ovine follicle stimulating hormone, by Pichia pastoris.
Authors:Fidler AE, Lun S, Young W, McNatty KP
Journal:J Mol Endocrinol
PubMed ID:9845673
'The methylotrophic yeast, Pichia pastoris, has been used to co-express recombinant genes formed by fusion of the mating factor-alpha (MFalpha) leader and ovine follicle stimulating hormone (oFSH) alpha and beta subunit coding sequences. Pichia strains carrying single copies of the two fusion genes secreted recombinant oFSH (roFSH) to concentrations of ... More
Improved tumour targeting by disulphide stabilized diabodies expressed in Pichia pastoris.
Authors:FitzGerald K, Holliger P, Winter G,
Journal:Protein Eng
PubMed ID:9488147
'Diabodies are dimeric antibody fragments held together by associated heavy and light chain variable domains present on different polypeptide chains. To improve their stability we have introduced cysteine residues into the V-domains to promote the disulphide crosslinking of the dimer. A crosslinked bivalent diabody against carcinoembryonic antigen (CEA) and a ... More
High-level expression of recombinant Aplysia ADP-ribosyl cyclase in offhia pastoris by fermentation.
Authors:Munshi C, Lee HC
Journal:Protein Expr Purif
PubMed ID:9325145
'Cyclic ADP-ribose (cADPR), a Ca2+ mobilizing cyclic nucleotide derived from NAD+, is rapidly emerging as an endogenous modulator of Ca2(+)- induced Ca2+ release mechanisms in various cellular systems. ADP ribosyl cyclase, first isolated from the marine invertebrate Aplysia californica, cyclizes NAD+ to cADPR. In this study we have utilized the ... More
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