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基于蔗糖代谢关键基因的鉴定构建高效生产透明质酸的兽疫链球菌菌株。

Construction of efficient Streptococcus zooepidemicus strains for hyaluoronic acid production based on identification of key genes involved in sucrose metabolism.

作者信息

Zhang Xuzhen, Wang Man, Li Tuanjie, Fu Lixia, Cao Wei, Liu Hao

机构信息

MOE Key Lab of Industrial Fermentation Microbiology, College of Biotechnology, Tianjin University of Science & Technology, Tianjin, 300457, China.

出版信息

AMB Express. 2016 Dec;6(1):121. doi: 10.1186/s13568-016-0296-7. Epub 2016 Nov 28.

Abstract

Biosynthesis of polysaccharide hyaluoronic acid (HA) by Streptococcus zooepidemicus is a carbon-intensive process. The carbon flux and factor(s) restricting HA yield were not well understood. Here, we investigated the function of genes involved in sucrose metabolism and identified targets limiting HA yield, which were exploited to construct efficient S. zooepidemicus strains for HA production. The sucrose uptake was addressed by deletion of scrA and scrB, which encodes sucrose-PTS permease and sucrose-6-phosphate hydrolase, respectively. We found that scrB was essential for the growth of S. zooepidemicus and HA biosynthesis, and accumulation of sucrose-6-phosphate was toxic. ΔscrB could not grow in THY-sucrose medium, while ΔscrA and ΔscrAΔscrB showed negligible growth defects. Overexpression of scrA significantly reduced biomass and HA production, while overexpression of scrB resulted in 26% increase of biomass and 30% increase of HA yield. We revealed that fructose-6-phosphate for HA biosynthesis mainly originates from glucose-6-phosphate. Deletion of scrK, a gene encoding hexokinase, led to 11% reduction of biomass and 12% decrease of HA yield, while deletion of hasE, a gene encoding phosphoglucoisomerase, resulted in the abolishment of HA biosynthesis and a significantly slow growth. We found that HA biosynthesis could be improved by directing carbon flux to fructose-6-phosphate. Deletion of fruA encoding the EII of fructose-PTS and fruK encoding phosphofructokinase showed no apparent effect on cell growth, but resulted in 22 and 27% increase of HA yield, respectively. Finally, a strain with 55% increase of HA was constructed by overexpression of scrB in ΔfruK. These results provide a solid foundation for further metabolic engineering of S. zooepidemicus for highly efficient HA production.

摘要

兽疫链球菌合成多糖透明质酸(HA)是一个碳密集型过程。碳通量和限制HA产量的因素尚未得到充分了解。在此,我们研究了参与蔗糖代谢的基因功能,并确定了限制HA产量的靶点,利用这些靶点构建了用于HA生产的高效兽疫链球菌菌株。通过缺失分别编码蔗糖-PTS通透酶和蔗糖-6-磷酸水解酶的scrA和scrB来解决蔗糖摄取问题。我们发现scrB对兽疫链球菌的生长和HA生物合成至关重要,蔗糖-6-磷酸的积累具有毒性。ΔscrB在THY-蔗糖培养基中无法生长,而ΔscrA和ΔscrAΔscrB显示出可忽略不计的生长缺陷。scrA的过表达显著降低了生物量和HA产量,而scrB的过表达导致生物量增加26%,HA产量增加30%。我们发现用于HA生物合成的6-磷酸果糖主要源自6-磷酸葡萄糖。缺失编码己糖激酶的scrK导致生物量减少11%,HA产量降低12%,而缺失编码磷酸葡萄糖异构酶的hasE导致HA生物合成停止且生长显著缓慢。我们发现通过将碳通量导向6-磷酸果糖可以提高HA生物合成。缺失编码果糖-PTS EII的fruA和编码磷酸果糖激酶的fruK对细胞生长没有明显影响,但分别导致HA产量增加22%和27%。最后,通过在ΔfruK中过表达scrB构建了一株HA产量提高55%的菌株。这些结果为进一步对兽疫链球菌进行代谢工程改造以实现高效HA生产提供了坚实基础。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6f2f/5125315/b82ffeb046eb/13568_2016_296_Fig1_HTML.jpg

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