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Expression and characterization of antimicrobial peptides Retrocyclin‐101 and Protegrin‐1 in chloroplasts to control viral and bacterial infections

机译:抗微生物肽逆转晶蛋白-101和protegrin-1在叶绿体中治疗病毒和细菌感染的表达及表征

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Summary Retrocyclin-101 (RC101) and Protegrin-1 (PG1) are two important antimicrobial peptides that can be used as therapeutic agents against bacterial and/or viral infections, especially those caused by the HIV-1 or sexually transmitted bacteria. Because of their antimicrobial activity and complex secondary structures, they have not yet been produced in microbial systems and their chemical synthesis is prohibitively expensive. Therefore, we created chloroplast transformation vectors with the RC101 or PG1 coding sequence, fused with GFP to confer stability, furin or Factor Xa cleavage site to liberate the mature peptide from their fusion proteins and a His-tag to aid in their purification. Stable integration of RC101 into the tobacco chloroplast genome and homoplasmy were confirmed by Southern blots. RC101 and PG1 accumulated up to 32%–38% and 17%∼26% of the total soluble protein. Both RC101 and PG1 were cleaved from GFP by corresponding proteases in vitro , and Factor Xa–like protease activity was observed within chloroplasts. Confocal microscopy studies showed location of GFP fluorescence within chloroplasts. Organic extraction resulted in 10.6-fold higher yield of RC101 than purification by affinity chromatography using His-tag. In planta bioassays with Erwinia carotovora confirmed the antibacterial activity of RC101 and PG1 expressed in chloroplasts. RC101 transplastomic plants were resistant to tobacco mosaic virus infections, confirming antiviral activity. Because RC101 and PG1 have not yet been produced in other cell culture or microbial systems, chloroplasts can be used as bioreactors for producing these proteins. Adequate yield of purified antimicrobial peptides from transplastomic plants should facilitate further preclinical studies.
机译:发明内容核霉素-101(RC101)和protegrin-1(PG1)是两种重要的抗微生物肽,其可用作免受细菌和/或病毒感染的治疗剂,尤其是由HIV-1或性传播的细菌引起的那些。由于它们的抗微生物活性和复杂的二级结构,它们尚未在微生物系统中产生,并且它们的化学合成是昂贵的。因此,我们用RC101或PG1编码序列创建了叶绿体转化载体,与GFP融合以赋予稳定性,Furin或因子Xa切割位点以从它们的融合蛋白和His-标签释放成熟肽以帮助其纯化。通过Southern印迹确认RC101稳定地整合RC101进入烟草基因组和同源性。 RC101和PG1累积高达总可溶性蛋白质的32%-38%和17%〜26%。将RC101和PG1从体外相应的蛋白酶从GFP切割,并且在叶绿体中观察到因子XA样蛋白酶活性。共聚焦显微镜研究显示GFP荧光在叶绿体中的位置。有机萃取产生的RC101的产率为10.6倍,而不是通过HIS-TAG纯化。在血管生物测定中,埃尔维亚Carotovora证实了在叶绿体中表达的RC101和PG1的抗菌活性。 RC101移植剂植物对烟草叶片病毒感染有抗性,确认抗病毒活性。因为RC101和PG1尚未在其他细胞培养物或微生物系统中产生,所以叶绿体可以用作用于生产这些蛋白质的生物反应器。来自移植体植物的纯化抗微生物肽的足够产量应促进进一步的临床前研究。

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