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Identification of a novel promoter for driving antibiotic-resistant genes to reduce the metabolic burden during protein expression and effectively select multiple integrations in Pichia Pastoris

Appl Microbiol Biotechnol. 2021-04; 
Qi Shen, Zhuang Yu, Xiao-Ting Zhou, Shi-Jia Zhang, Shu-Ping Zou, Neng Xiong, Ya-Ping Xue, Zhi-Qiang Liu, Yu-Guo Zheng
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Proteins, Expression, Isolation and Analysis Twenty micrograms of cytosolic proteins determined by the BCA assay (Biyotime, Shanghai, China) was subjected to 4–12% GenScript SurePAGE gel (Nanjing, China) Get A Quote

摘要

Routine approaches for the efficient expression of heterogenous proteins in Pichia pastoris include using the strong methanol-regulated alcohol oxidase (AOX1) promoter and multiple inserts of expression cassettes. To screen the transformants harboring multiple integrations, antibiotic-resistant genes such as the Streptoalloteichus hindustanus bleomycin gene are constructed into expression vectors, given that higher numbers of insertions of antibiotic-resistant genes on the expression vector confer resistance to higher concentrations of the antibiotic for transformants. The antibiotic-resistant genes are normally driven by the strong constitutive translational elongation factor 1a promoter (P). However, antibiot... More

關鍵詞

Antibiotic-resistant gene, Glucose-regulated promoter, Pichia pastoris, Promoter, Zeocin
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