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通过对共生甲藻微小共生藻(Symbiodinium minutum)的基因组调查鉴定出的多功能聚酮合酶基因。

Multifunctional polyketide synthase genes identified by genomic survey of the symbiotic dinoflagellate, Symbiodinium minutum.

作者信息

Beedessee Girish, Hisata Kanako, Roy Michael C, Satoh Noriyuki, Shoguchi Eiichi

机构信息

Marine Genomics Unit, Okinawa Institute of Science and Technology Graduate University, Onna, Okinawa, 904-0495, Japan.

Imaging and Instrumental Analysis Section, Okinawa Institute of Science and Technology Graduate University, Onna, Okinawa, 904-0495, Japan.

出版信息

BMC Genomics. 2015 Nov 14;16:941. doi: 10.1186/s12864-015-2195-8.

Abstract

BACKGROUND

Dinoflagellates are unicellular marine and freshwater eukaryotes. They possess large nuclear genomes (1.5-245 gigabases) and produce structurally unique and biologically active polyketide secondary metabolites. Although polyketide biosynthesis is well studied in terrestrial and freshwater organisms, only recently have dinoflagellate polyketides been investigated. Transcriptomic analyses have characterized dinoflagellate polyketide synthase genes having single domains. The Genus Symbiodinium, with a comparatively small genome, is a group of major coral symbionts, and the S. minutum nuclear genome has been decoded.

RESULTS

The present survey investigated the assembled S. minutum genome and identified 25 candidate polyketide synthase (PKS) genes that encode proteins with mono- and multifunctional domains. Predicted proteins retain functionally important amino acids in the catalytic ketosynthase (KS) domain. Molecular phylogenetic analyses of KS domains form a clade in which S. minutum domains cluster within the protist Type I PKS clade with those of other dinoflagellates and other eukaryotes. Single-domain PKS genes are likely expanded in dinoflagellate lineage. Two PKS genes of bacterial origin are found in the S. minutum genome. Interestingly, the largest enzyme is likely expressed as a hybrid non-ribosomal peptide synthetase-polyketide synthase (NRPS-PKS) assembly of 10,601 amino acids, containing NRPS and PKS modules and a thioesterase (TE) domain. We also found intron-rich genes with the minimal set of catalytic domains needed to produce polyketides. Ketosynthase (KS), acyltransferase (AT), and acyl carrier protein (ACP) along with other optional domains are present. Mapping of transcripts to the genome with the dinoflagellate-specific spliced leader sequence, supports expression of multifunctional PKS genes. Metabolite profiling of cultured S. minutum confirmed production of zooxanthellamide D, a polyhydroxy amide polyketide and other unknown polyketide secondary metabolites.

CONCLUSION

This genomic survey demonstrates that S. minutum contains genes with the minimal set of catalytic domains needed to produce polyketides and provides evidence of the modular nature of Type I PKS, unlike monofunctional Type I PKS from other dinoflagellates. In addition, our study suggests that diversification of dinoflagellate PKS genes comprises dinoflagellate-specific PKS genes with single domains, multifunctional PKS genes with KS domains orthologous to those of other protists, and PKS genes of bacterial origin.

摘要

背景

甲藻是单细胞海洋和淡水真核生物。它们拥有庞大的核基因组(1.5 - 245千兆碱基),并产生结构独特且具有生物活性的聚酮类次生代谢产物。尽管聚酮生物合成在陆地和淡水生物中已得到充分研究,但直到最近才开始对甲藻聚酮进行研究。转录组分析已经鉴定出具有单个结构域的甲藻聚酮合酶基因。共生藻属基因组相对较小,是一组主要的珊瑚共生体,微小共生藻的核基因组已被解码。

结果

本研究调查了组装后的微小共生藻基因组,鉴定出25个候选聚酮合酶(PKS)基因,这些基因编码具有单功能和多功能结构域的蛋白质。预测的蛋白质在催化酮合成酶(KS)结构域中保留了功能重要的氨基酸。对KS结构域的分子系统发育分析形成了一个进化枝,其中微小共生藻的结构域与其他甲藻和其他真核生物的结构域聚集在原生生物I型PKS进化枝内。单结构域PKS基因可能在甲藻谱系中得到了扩展。在微小共生藻基因组中发现了两个源于细菌的PKS基因。有趣的是,最大的酶可能以一种由10,601个氨基酸组成的杂合非核糖体肽合成酶 - 聚酮合酶(NRPS - PKS)组装形式表达,包含NRPS和PKS模块以及一个硫酯酶(TE)结构域。我们还发现了富含内含子的基因,这些基因具有产生聚酮所需的最少催化结构域集。酮合成酶(KS)、酰基转移酶(AT)和酰基载体蛋白(ACP)以及其他可选结构域均存在。利用甲藻特异性剪接前导序列将转录本映射到基因组上,支持了多功能PKS基因的表达。对培养的微小共生藻进行代谢物谱分析,证实了虫黄藻酰胺D(一种多羟基酰胺聚酮)和其他未知聚酮次生代谢产物的产生。

结论

这项基因组研究表明,微小共生藻含有产生聚酮所需的最少催化结构域集的基因,并提供了I型PKS模块化性质的证据,这与其他甲藻的单功能I型PKS不同。此外,我们的研究表明,甲藻PKS基因的多样化包括具有单个结构域的甲藻特异性PKS基因、与其他原生生物KS结构域直系同源的多功能PKS基因以及源于细菌的PKS基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8b23/4647583/1c860f3d18c0/12864_2015_2195_Fig1_HTML.jpg

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