Optimization of the expression of recombinant human activin A in the yeast <i>Pichia pastoris</i>

Fredericks, Dale Patricia; Clay, Robert L.; Warner, Tracy; O’Connor, Anne E; Kretser, David de; Hearn, Milton Thomas William

doi:10.1002/btpr.304

Cited by 11 publications

(9 citation statements)

References 65 publications

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“…There are several reports of the overexpression of mammalian signaling proteins in non-mammalian cells, including human BMP-2, bovine activin A, and bovine inhibin A in insect cells [42,43] and human activin A in yeast [44]. These expression hosts have some advantages over mammalian cells, including the absence of native binding partners that can interfere with maturation [18] and potentially higher yields [44,45]. The higher yields have only been obtained when the protease cleavage site between the pro-domain and mature signaling dimer have been altered to more closely match the endogenous proteases in the expression host [44,45].…”

Section: Methodsmentioning

confidence: 99%

“…These expression hosts have some advantages over mammalian cells, including the absence of native binding partners that can interfere with maturation [18] and potentially higher yields [44,45]. The higher yields have only been obtained when the protease cleavage site between the pro-domain and mature signaling dimer have been altered to more closely match the endogenous proteases in the expression host [44,45]. Thus, successful heterologous expression has required some alterations to account for differences in molecular machinery relative to mammalian hosts, but so far these have been relegated to the enzymes responsible for proteolytic processing, not enzymes involved in catalyzing disulfide exchange or folding.…”

Section: Methodsmentioning

confidence: 99%

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Production, Isolation, and Structural Analysis of Ligands and Receptors of the TGF-β Superfamily

Huang

Hinck²

2016

Methods in Molecular Biology

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The ability to understand the molecular mechanisms by which secreted signaling proteins of the TGF-β superfamily assemble their cell surface receptors into complexes to initiate downstream signaling is dependent upon the ability to determine atomic-resolution structures of the signaling proteins, the ectodomains of the receptors, and the complexes that they form. The structures determined to date have revealed major differences in the overall architecture of the signaling complexes formed by the TGF-βs and BMPs, which has provided insights as to how they have evolved to fulfill their distinct functions. Such studies, have however, only been applied to a few members of the TGF-β superfamily, which is largely due to the difficulty of obtaining milligram-scale quantities of highly homogenous preparations of the disulfide-rich signaling proteins and receptor ectodomains of the superfamily. Here we describe methods used to produce signaling proteins and receptor ectodomains of the TGF-β superfamily using bacterial and mammalian expression systems and procedures to purify them to homogeneity.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Production, Isolation, and Structural Analysis of Ligands and Receptors of the TGF-β Superfamily

Huang

Hinck²

2016

Methods in Molecular Biology

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“…In the simplest method, one can optimize conditions of the culture such as culture medium, cell density, inducer concentration, temperature, pH, aeration, etc. (Maldonado et al 2007;Maldonado et al 2008;Zhao et al 2008;Fredericks et al 2010;Varghese et al 2010). However, most of the time, improving external factors is not sufficient, whereas changing some genetic factors can significantly impact the production of recombinant protein Li et al 2008).…”

Section: Introductionmentioning

confidence: 98%

Elevating the expression level of biologically active recombinant human alpha 1-antitrypsin in Pichia pastorisan alpha 1-antitrypsin in Pichia pastoris

Arjmand¹,

Lotfi²,

Shamsara³

et al. 2013

Electron. J. Biotechnol.

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Background: Human alpha 1-antitrypsin (AAT) is a potent inhibitor of multiple serine proteases, and protects tissues against their harmful effects. Individuals with reduced or abnormal production of this inhibitor need intravenous administration of exogenous protein. In this study, we employed the methylotrophic (methanol utilizing) yeast Pichia pastoris (P. pastoris) as a preferential host for efficient production and secretion of recombinant AAT. Furthermore, we examined different strategies to maximize the yield of the secreted protein.Results: Our findings revealed that optimizing the codon usage of AAT gene for P. pastoris had positive effects on the level of secreted AAT under the control of inducible alcohol oxidase 1 (AOX1) and constitutive glycerol aldehyde phosphate dehydrogenase (GAP) promoters. Compared to AOX1, the GAP promoter increased the yield of AAT by more than two fold. It was also demonstrated that the human AAT native signal sequence was more effective than the well-known yeast signal sequence, alpha mating factor (α-MF). Doubling gene dosage nearly doubled the production of AAT, though dosages exceeding this limit had negative effects on the yield. Conclusion: P. pastoris is shown to be an efficient expression system for production of recombinant and biologically active AAT. Also different strategies could be used to elevate the amount of this secretable protein.

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“…The recombinant plasmid, pPICZ B‐M f (10 μg) was linearized using Sac I and introduced into P. pastoris X33 strain via electroporation (Micropulser, BioRad, Hercules, CA) at 2 kV for ∼5 ms as described by Fredericks et al After transformation, the yeast cells were plated on the Yeast Extract Peptone Dextrose agar containing zeocin (100 μg/mL; Invitrogen, USA). In order to select for clones with higher resistance level, transformants were plated on Yeast Extract Peptone Dextrose agar containing increasing concentration of zeocin (250, 500, and 1,000 μg/mL).…”

Section: Methodsmentioning

confidence: 99%

Production of the virus‐like particles of nipah virus matrix protein in Pichia pastoris as diagnostic reagents

Joseph

Tey

et al. 2016

Biotechnology Progress

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The matrix (M) protein of Nipah virus (NiV) is a peripheral protein that plays a vital role in the envelopment of nucleocapsid protein and acts as a bridge between the viral surface and the nucleocapsid proteins. The M protein is also proven to play an important role in production of virus-like particles (VLPs) and is essential for assembly and budding of NiV particles. The recombinant M protein produced in Escherichia coli assembled into VLPs in the absence of the viral surface proteins. However, the E. coli produced VLPs are smaller than the native virus particles. Therefore, the aims of this study were to produce NiV M protein in Pichia pastoris, to examine the structure of the VLPs formed, and to assess the potential of the VLPs as a diagnostic reagent. The M protein was successfully expressed in P. pastoris and was detected with anti-myc antibody using Western blotting. The VLPs formed by the recombinant M protein were purified with sucrose density gradient ultracentrifugation, high-performance liquid chromatography (HPLC), and Immobilized Metal Affinity Chromatography (IMAC). Immunogold staining and transmission electron microscopy confirmed that the M protein assembled into VLPs as large as 200 nm. ELISA revealed that the NiV M protein produced in P. pastoris reacted strongly with positive NiV sera demonstrating its potential as a diagnostic reagent. © 2016 American Institute of Chemical Engineers Biotechnol. Prog., 32:1038-1045, 2016.

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Optimization of the expression of recombinant human activin A in the yeast Pichia pastoris

Cited by 11 publications

References 65 publications

Production, Isolation, and Structural Analysis of Ligands and Receptors of the TGF-β Superfamily

Production, Isolation, and Structural Analysis of Ligands and Receptors of the TGF-β Superfamily

Elevating the expression level of biologically active recombinant human alpha 1-antitrypsin in Pichia pastorisan alpha 1-antitrypsin in Pichia pastoris

Production of the virus‐like particles of nipah virus matrix protein in Pichia pastoris as diagnostic reagents

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