1.Construction of a Pichia pastoris recombinant strain capable of over-expressing phytase and endoglucanase.
Zhenfang WU ; Zizhong TANG ; Hui CHEN ; Xueyi HAN ; Xin LAI ; Qi WU
Chinese Journal of Biotechnology 2010;26(5):616-622
Both phytase and endoglucanase are additives in feed for mono-gastric animal known for their effects. Recombinant vector pPICZalpha-EG was constructed and transformed to GS115-phyA, a Pichia pastoris strain that had integrated with phytase gene, generating GS115-phyA-EG. Both phytase and endoglucanase activities in the supernatant were determined after methanol induction of GS115-phyA-EG. Phytase and endoglucanase activity reached 39.4% and 56.2% activity compared to GS115-phyA and GS115-EG, respectively. Properties of the mixed enzyme suggest that the optimal temperature and pH value be 55 degrees C and 5.5 respectively. Both phytase and endoglucanase showed greater than 80% activity across temperature ranges 45 degrees C to 55 degrees C and pH ranges 4.5 to 5.5. Expressing more than one enzyme in one system could save time and money during induced expression, and the mixed enzyme might apply for treating forge before feeding with poultry.
6-Phytase
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biosynthesis
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genetics
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Cellulase
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biosynthesis
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genetics
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Genetic Vectors
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Pichia
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enzymology
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genetics
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Recombinant Proteins
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biosynthesis
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genetics
2.The analysis of heterogeneity of HWTX-I expressed in Pichia pastoris.
Dong-Song NIE ; Yan-Kai ZHOU ; Zuo-Ying CAO ; Yu LIU
Chinese Journal of Biotechnology 2006;22(2):215-219
To seek the reason of heterogeneity of recombinant HWTX-I (rHWTX-I) expressed in Pichia pastoris. We expressed HWTX-I gene of interest in Pichia pastoris GS115/HWTX-I. The heterogenous product expressed was separated, purified and identified by using Ion exchange HPLC, reverse HPLC, Tricine SDS-PAGE and MALDI-TOF Mass Spectrometry and then sequenced in both N-terminus and C-terminus. These results show that the heterogeneity of rHWTX-I results from the incomplete processing of signal peptide of N-terminus and the internal degradation of C-terminus. Biological activity assay shows that the activity of the heterogenous rHWTX-I only showed 30% activity compared with the native HWTX-I. The Solutions to how to avoid the heterogeneity are also discussed.
Animals
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Neurotoxins
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biosynthesis
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genetics
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Pichia
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genetics
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metabolism
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Recombinant Proteins
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biosynthesis
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genetics
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Reptilian Proteins
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biosynthesis
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genetics
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Spider Venoms
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biosynthesis
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genetics
3.Optimization of plant des-pGlu1-Brazzein gene according to yeasty biased codons and its expression in Pichia pastoris.
Chunli LI ; Lu HAN ; Zhenyu ZHENG ; Weidong ZHAO
Chinese Journal of Biotechnology 2011;27(8):1158-1163
According to the amino acid sequence of des-pGlu1-Brazzein, 4 pairs of oligonucleotide with cosmic site were synthesized by using yeasty biased codons. After linkage and PCR, the 179 bp code area of des-pGlu1-Brazzein was obtained and inserted into pPIC9K, which resulted in the recombinant expression vector pPIC9K-Bra. By digestion with Sal I, the lined pPIC9K-Bra was transformed into Pichia pastoris GS115 by electric shock. The results of expression indicted that the secreted target protein accounted for 51.6% of total protein in the supernatant and showed biological activity after purification.
Codon
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Pichia
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genetics
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metabolism
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Plant Proteins
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biosynthesis
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genetics
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Recombinant Proteins
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biosynthesis
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genetics
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isolation & purification
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Sweetening Agents
4.Overexpression of a sweet protein monellin in Escherichia coli.
Zhong-Jun CHEN ; Heng CAI ; Fu-Ping LU ; Lian-Xiang DU
Chinese Journal of Biotechnology 2005;21(4):568-572
According to the amino acid sequence of monellin, a single chain 294bp monellin gene was synthesized and inserted into vector pET-22b to yield the recombinant secretion plasmid pETMO. The single-chain monellin gene was designed based on the biased codons of E. coli so that its expression would be then optimized. Under the expressing conditions, monellin was produced accounting for 44.8% of total soluble proteins. The E. coli-expressed single-chain monellin is 3000 times sweeter than sucrose. The thermal-stability and acid-resistance of the protein are higher than the natural monellin.
Escherichia coli
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genetics
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metabolism
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Plant Proteins
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biosynthesis
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genetics
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Protein Engineering
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methods
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Recombinant Proteins
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biosynthesis
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genetics
5.Effect of mutating subsite -7 on product specificity of cyclodextrin glucanotransferase from alkalophilic Bacillus clarkii.
Dong YANG ; Jingfei TIAN ; Sheng CHEN ; Jing WU
Chinese Journal of Biotechnology 2012;28(2):191-202
To investigate the mechanism of high product specificity of gamma-clodextrin glucanotransferase (CGTase) from alkalophilic Bacillus clarkii 7364, we aligned protein sequence and structure model, found out that loss of 6 amino acids at subsite -7 probably affected its product specificity. Using overlapping PCR method, we inserted 6 amino acids into subsite -7 of CGTase. The mutant CGTase gene was ligated with pET-20b (+) and expressed in Escherichia coli BL21 (DE3). The extracellular recombinant enzyme was used to transform soluble starch into cyclodextrins (CDs). HPLC analysis results show that, compared to wild CGTase, the gamma-CDs produced by mutant enzyme decreased from 76.0% to 12.5%, whereas the ratio of alpha- and beta-CDs increased from 8.7% and 15.2% to 37.5% and 50%. The possible mechanism was that, compared to alpha-, beta-CGTase, wild gamma-CGTase lacks 6 amino acids in its subsite -7. This conformation provided more space for glucose combination and was thus advantageous for forming gamma-CD. When the 6 amino acids were inserted into the subsite -7 of wild gamma-CGTase, the space to bind with glucose reduced and consequently resulted in less gamma-CD production.
Bacillus
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enzymology
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genetics
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Escherichia coli
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genetics
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metabolism
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Glucosyltransferases
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biosynthesis
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genetics
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Mutant Proteins
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biosynthesis
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genetics
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Recombinant Proteins
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biosynthesis
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genetics
6.Secreted expression of porcine interferon-gamma gene in Pichia pastoris.
Zhi-Qing HUANG ; Hong-Yu HU ; Xiao-Ling CHEN ; Li-Ming REN ; Ai-Xing LIN ; Yong-Fu CHEN
Chinese Journal of Biotechnology 2005;21(5):731-736
The porcine interferon-gamma (PoIFN-gamma) gene, in which the sequence encoding signal peptide was replaced by that of the alpha-factor of Saccharomyces cerevisiae, was cloned into Pichia pastoris expression vector pPIC9K. The recombinant plasmid pPIC9K-alpha-PoIFN-gamma was then transformed into Pichia pastoris GS115 cells by electroporation and stable multicopy recombinant Pichia pastoris strains were selected by G418 resistance. Two recombinants of multiple inserts were obtained. SDS-PAGE and Western blot assays of culture broth from a methanol-induced expression strain demonstrated that recombinant PoIFN-gamma, 17kD and 23kD proteins, were secreted into the culture medium. Target proteins, 60% of total proteins, were obtained in the culture medium at the concentration of 108 mg/L. This is the first secreted expression of porcine interferon-gamma gene in Pichia pastoris.
Animals
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Electroporation
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Interferon-gamma
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biosynthesis
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genetics
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Pichia
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genetics
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metabolism
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Recombinant Proteins
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biosynthesis
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genetics
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Swine
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genetics
7.Expression and analysis of the recombinant human interleukin-21 (rhIL-21) in Pichia pastoris.
Dong LI ; Huiqing YU ; Rongfen HUO ; Jianquan CHEN ; Guoxiang CHENG
Chinese Journal of Biotechnology 2009;25(11):1711-1717
Interleukin-21 is a type I cytokine mainly produced by activated CD4+ T cells that acts as a regulator of immune system. In this work, hIL-21cDNA was amplified from human peripheral blood lymphocytes by RT-PCR, and then inserted into pPIC9K. The recombinant vector pPIC9K-hIL21cDNA was linearized by Sac I, and transformed into Pichia pastoris strain GS115 by electroporation. Transformants were selected by G418 and confirmed by PCR. The recombinant protein was expressed and secreted into the supernatant after inducing by methanol. SDS-PAGE analysis indicated the molecular weight of rhIL-21 was about 16 kD. ELISA results show that the yield of rhIL-21 reach 229.28 mg/L, rhIL-21 was purified from culture supernatants, and it was purified to about 95% purity with ion-exchange chromatography. When co-stimulate with Con A, rhIL-21 can promote the proliferation of human lymphocytes. This is the first expression of bio-active rhIL-21 in Pichia pastoris. It lays a foundation for further research in immunotherapy and cancer therapy.
Electroporation
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Genetic Vectors
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genetics
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Humans
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Interleukins
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biosynthesis
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genetics
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Pichia
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genetics
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metabolism
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Recombinant Proteins
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analysis
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biosynthesis
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genetics
8.Expression of Vitreoscilla hemoglobin improves recombinant lipase production in Pichia pastoris.
Xiaofeng WANG ; Yongchuan SUN ; Xuguang SHEN ; Feng KE ; Li XU ; Yun LIU ; Yunjun YAN
Chinese Journal of Biotechnology 2011;27(12):1755-1764
Yarrowia lipolytica lipase Lip2 (YlLip2) is an important industrial enzyme with many potential applications. To alleviate the dissolved oxygen (DO) limitation and improve YlLip2 production during high-cell density fermentation, the YlLip2 gene lip2 and Vitreoscilla hemoglobin (VHb) gene vgb were co-expressed in Pichiapastoris under the control of AOX1 and PsADH2 promoter, respectively. The PsADH2 promoter from Pichia stipitis could be activated under oxygen limitation. The SDS-PAGE and CO-difference spectrum analysis indicated that VHb and YlLip2 had successfully co-expressed in recombinant strains. Compared with the control cells (VHb-, GS115/9Klip2), the expression levels of YlLip2 in VHb-expressing cells (VHb+, GS115/9Klip2-pZPVT) under oxygen limitation were improved 25% in shake-flask culture and 83% in a 10 L fermentor. Moreover, the VHb+ cells displayed higher biomass than VHb- cells at lower DO levels in a 10 L fermentor. In this study, we also achieved a VHb-expressing clone harboring multicopy lip2 gene (GS115/9Klip2-pZPVTlip2 49#), which showed the maximum lipolytic activity of 33 900 U/mL in a 10 L fermentor under lower DO conditions. Therefore, it can be seen that expression of VHb with PsADH2 promoter in P. pastoris combined with increasing copies of lip2 gene is an effective strategy to improve YlLip2 production.
Bacterial Proteins
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biosynthesis
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genetics
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Fermentation
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Fungal Proteins
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biosynthesis
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genetics
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Lipase
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biosynthesis
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genetics
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Oxygen
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analysis
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pharmacology
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Pichia
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metabolism
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Protein Engineering
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Recombinant Proteins
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biosynthesis
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genetics
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Truncated Hemoglobins
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biosynthesis
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genetics
9.Soluble expression of recombinant human apoliprotein A-I-Milano in Escherichia coli.
Ming LI ; Hong-Liang ZHAO ; Chong XUE ; Wei ZHANG ; Shi-Meng ZHANG ; Zhi-Min LIU
Chinese Journal of Biotechnology 2005;21(3):354-359
Apolipoprotein A-I-Milano(AIM), a natural variant, not only inhibits the initiation and progression of atherosclerosis, but also makes the preexisting atherosclerotic lesions regress. AIM gene, at which N-terminal codens were optimized, was subcloned into the expression vector of pET22b. Recombiant plasmids were transformed into E. coli strain BL21 (DE3) and induced with IPTG. The expressed apoliprotein A-I-Milano was soluble in E. coli and was about 38% of total cell lysate. Purified by Butyl Sepharose 4F. F hydrophobic chromatography and Q Sepharose H.P. anion exchange chromatography, followed by ultrafiltration with Vivaspin 20 (30 000MW), AIM monomer was obtained in a purity of more than 95%. Activity assay of binding of AIM monomer to lipid indicates that association of AIM monomer with DMPC is slower than normal apoA-I but DMPC number associated by AIM monomer is more than by apoA-I. This results will be important for studying structure, function of AIM, specially clinical application.
Apolipoprotein A-I
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biosynthesis
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genetics
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Escherichia coli
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genetics
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metabolism
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Humans
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Mutant Proteins
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biosynthesis
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genetics
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Recombinant Proteins
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biosynthesis
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genetics
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Solubility
10.Identification and expression patterns of anterior silk gland specific cuticle protein Bm11721 in the silkworm (Bombyx mori).
Kang XIE ; Xin WANG ; Huifang CHEN ; Yi LI ; Qianru SONG ; Ping ZHAO
Chinese Journal of Biotechnology 2016;32(1):64-73
The silk gland of silkworm is the organ of silk protein synthesis and secretion. According to the morphological and functional differences, silk gland can be divided into anterior silk gland (ASG), middle silk gland (MSG) and posterior silk gland (PSG). ASG is the place for silk proteins conformation changes although it cannot synthetize silk proteins. ASG has narrow luminal structures and rigid wall which consists of chitin and cuticle proteins so that it can provide the shearing force which plays an important role in the silk protein conformation changes. The objective of this study is to identify the new chitin binding proteins in ASG of silkworm (Bombyx mori), and to analyze their expression patterns in different tissues. We identified a cuticle protein with chitin binding domain Bml1721 (GenBank Accession No. NM-001173285.1) by chitin affinity chromatography column. We also expressed the recombinant protein as inclusion body using the prokaryotic expression system, and then successfully purified the recombinant protein by nickel affinity chromatography column to generate the polyclonal antibodies. The expression patterns analysis in various tissues showed that both in transcriptional and protein levels Bm11721 was specifically expressed in ASG. Furthermore, the expression level of Bm 11721 protein was unchanged during the 5th instar. Immunofluorescence analysis revealed that Bm1 1721 was located in the ASG inner membrane. It is proposed that Bm11721 is a component of inner membrane and probably provides the shearing force for conformational changes.
Animals
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Bombyx
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genetics
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metabolism
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Chitin
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metabolism
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Insect Proteins
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genetics
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metabolism
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Recombinant Proteins
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biosynthesis
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Silk
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biosynthesis