Development and application of a droplet-based microfluidic high-throughput screening of Pichia pastoris.

Tong LÜ; Ran TU; Huiling Yuan; Hao Liu; Qinhong Wang

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Development and application of a droplet-based microfluidic high-throughput screening of Pichia pastoris.

Author: Tong LÜ ¹ ; Ran TU ² ; Huiling YUAN ² ; Hao LIU ¹ ; Qinhong WANG ²
Author Information

1. College of Biotechnology, Tianjin University of Science & Technology, Tianjin 300457, China.
2. Key Laboratory of Systems Microbial Biotechnology, Tianjin Institute of Industrial Biotechnology, Chinese Academy of Sciences, Tianjin 300308, China.
Publication Type:Journal Article
Keywords: Pichia pastoris; droplet microfluidics; heterologous protein expression; high-throughput screening; protein secretion; single cell
MeSH: Microfluidics; Mutagenesis; Pichia; Plasmids; Polymerase Chain Reaction; Recombinant Proteins
From: Chinese Journal of Biotechnology 2019;35(7):1317-1325
CountryChina
Language:Chinese
Abstract: Pichia pastoris is one of the most convenient and widely used heterologous protein expression systems. To further improve its ability to express heterologous proteins, we developed a high-throughput P. pastoris screening method based on droplet microfluidic and demonstrated the method by screening and obtaining mutants with enhanced xylanase expression and secretion abilities. We used PCR (Polymerase Chain Reaction) amplification to obtain a fusion fragment of xylanase xyn5 gene and green fluorescent protein gfp gene, and cloned this fragment into pPIC9K, the expression vector of Pichia pastoris, to construct the plasmid pPIC9K-xyn5-gfp that recombined the DNA fragments of xylanase and green fluorescent protein. After this plasmid entered P. pastoris GS115 by electroporation, the P. pastoris SG strain that could express xylanase and green fluorescent protein was obtained. The above-said strains were then mutagenized by atmospheric room temperature plasma and subsequently encapsulated to form single-cell droplets. After 24-hour cultivation of the droplets, microfluidic screening was carried out to obtain the mutant strain with high xylanase expression for further construction and screening of the next mutagenesis library. After five rounds of droplet microfluidic screening, a highly productive strain P. pastoris SG-m5 was obtained. The activity of the expressed xylanase was 149.17 U/mg, 300% higher than that of those expressed by the original strain SG. This strain's ability to secrete heterologous protein was 160% higher than that of the original strain. With a screening throughput of 100 000 strains per hour, the high-throughput P. pastoris screening system based on single-cell droplet microfluidic developed by the present study screens a library with million strains in only 10 hours and consumes only 100 μL of fluorescent reagent, thus reducing the reagent cost by millions of times compared with the traditional microplate screening and more importantly, providing a novel method to obtain P. pastoris with high abilities to express and secret heterologous proteins by efficient and low-cost screening.