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溶组织内阿米巴的焦磷酸依赖性磷酸果糖激酶:分子克隆、重组表达及焦磷酸类似物的抑制作用

Pyrophosphate-dependent phosphofructokinase of Entamoeba histolytica: molecular cloning, recombinant expression and inhibition by pyrophosphate analogues.

作者信息

Bruchhaus I, Jacobs T, Denart M, Tannich E

机构信息

Bernhard Nocht Institute for Tropical Medicine, Hamburg, Federal Republic of Germany.

出版信息

Biochem J. 1996 May 15;316 ( Pt 1)(Pt 1):57-63. doi: 10.1042/bj3160057.

DOI:10.1042/bj3160057
PMID:8645233
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1217350/
Abstract

By using oligonucleotide primers derived from regions highly conserved in prokaryotic and eukaryotic phosphofructokinase sequences, a genomic DNA fragment was amplified and used to isolate cDNA and genomic clones coding for PPi-dependent phosphofructokinase (PPi-PFK) of Entamoeba histolytica. The open reading frame consists of 1308 bp and the corresponding protein has a calculated molecular mass of 47.6 kDa. The N-terminal half of the protein shows 27-35% identity with PPi-PFKs or ATP-dependent phosphofructokinases (ATP-PFKs) of various eukaryotic and prokaryotic organisms. The amino acid residues that form the active site of the PPi-PFK from Propionibacterium freudenreichii and the allosteric ATP-PFK from Escherichia coli are conserved within the amoeba sequence. The PPi-PFK was recombinantly expressed by using a prokaryotic expression system. The purified recombinant protein was found to be enzymically active. The K(m) values for PPi and fructose 6-phosphate of the native and the recombinant PPi-PFKs were nearly identical. Various bisphosphonates (synthetic pyrophosphate analogues) were tested for their ability to inhibit PPi-PFK activity or amoebic growth. All bisphosphonates tested were competitive inhibitors for amoeba PPi-PFK activity. The best inhibitors were CGP 48048 and zoledronate, with Ki values of 50 microM. All bisphosphonates inhibited amoebic growth. One of them (risedronate) was inhibitory at a concentration of 10 microM. Bisphosphonates are therefore potential therapeutic agents for the treatment of amoebiasis.

摘要

通过使用源自原核生物和真核生物磷酸果糖激酶序列中高度保守区域的寡核苷酸引物,扩增出一个基因组DNA片段,并用于分离编码溶组织内阿米巴焦磷酸依赖性磷酸果糖激酶(PPi-PFK)的cDNA和基因组克隆。开放阅读框由1308个碱基对组成,相应蛋白质的计算分子量为47.6 kDa。该蛋白质的N端一半与各种真核生物和原核生物的PPi-PFK或ATP依赖性磷酸果糖激酶(ATP-PFK)具有27%-35%的同一性。来自费氏丙酸杆菌的PPi-PFK和来自大肠杆菌的变构ATP-PFK的活性位点氨基酸残基在阿米巴序列中保守。通过使用原核表达系统重组表达PPi-PFK。发现纯化的重组蛋白具有酶活性。天然和重组PPi-PFK对PPi和6-磷酸果糖的K(m)值几乎相同。测试了各种双膦酸盐(合成焦磷酸类似物)抑制PPi-PFK活性或阿米巴生长的能力。所有测试的双膦酸盐都是阿米巴PPi-PFK活性的竞争性抑制剂。最佳抑制剂是CGP 48048和唑来膦酸盐,Ki值为50 microM。所有双膦酸盐均抑制阿米巴生长。其中一种(利塞膦酸盐)在浓度为10 microM时具有抑制作用。因此,双膦酸盐是治疗阿米巴病的潜在治疗药物。

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