首页> 美国卫生研究院文献>Proceedings of the Japan Academy. Series B Physical and Biological Sciences >Both the transglycosylase and transpeptidase functions in plastid penicillin-binding protein are essential for plastid division in Physcomitrella patens
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Both the transglycosylase and transpeptidase functions in plastid penicillin-binding protein are essential for plastid division in Physcomitrella patens

机译:质体青霉素结合蛋白中的转糖基化酶和转肽酶功能对于小立碗藓中质体的分裂都是必不可少的

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摘要

Class A penicillin-binding proteins (PBPs) are active in the final step of bacterial peptidoglycan biosynthesis. They possess a transglycosylase (TG) domain to polymerize the glycan chains and a transpeptidase (TP) domain to catalyze peptide cross-linking. We reported that knockout of the Pbp gene in the moss Physcomitrella patens (ΔPpPbp) results in a macrochloroplast phenotype by affecting plastid division. Here, expression of PpPBP-GFP in ΔPpPbp restored the wild-type phenotype and GFP fluorescence was observed mainly in the periphery of each chloroplast. Stable transformants expressing Anabaena PBP with the plastid-targeting sequence, or PpPBP replacing the Anabaena TP domain exhibited partial recovery, while chloroplast number was recovered to that of wild-type plants in the transformant expressing PpPBP replacing the Anabaena TG domain. Transient expression experiments with site-directed mutagenized PpPBP showed that mutations in the conserved amino acids in both domains interfered with phenotype recovery. These results suggest that both TG and TP functions are essential for function of PpPBP in moss chloroplast division.
机译:A类青霉素结合蛋白(PBP)在细菌肽聚糖生物合成的最终步骤中具有活性。它们具有转糖基化酶(TG)域以聚合聚糖链,并具有转肽酶(TP)域以催化肽交联。我们报道了在苔藓小立碗藓(Physcomitrella patens)(ΔPpPbp)中Pbp基因的敲除通过影响质体分裂而导致了大叶绿体表型。在此,ΔPpPbp中PpPBP-GFP的表达恢复了野生型表型,并且主要在每个叶绿体的外围观察到了GFP荧光。表达具有质体靶向序列的鱼腥藻PBP的稳定转化子,或替换鱼腥藻TP结构域的PpPBP表现出部分恢复,而在表达PpPBP替代鱼腥草TG结构域的转化子中,叶绿体的数量恢复到野生型植物的数量。用定点诱变的PpPBP进行的瞬时表达实验表明,两个结构域中保守氨基酸的突变均会干扰表型的恢复。这些结果表明,TG和TP功能对于PpPBP在苔藓叶绿体分裂中的功能至关重要。

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