Bayer A S, Coulter S N, Stover C K, Schwan W R
St. John's Cardiovascular Research Center, Division of Infectious Diseases, Harbor-UCLA Medical Center, Torrance, California 90509, USA.
Infect Immun. 1999 Feb;67(2):740-4. doi: 10.1128/IAI.67.2.740-744.1999.
Staphylococcus aureus causes a wide variety of invasive human infections. However, delineation of the genes which are essential for the in vivo survival of this pathogen has not been accomplished to date. Using signature tag mutagenesis techniques and large mutant pool screens, previous investigators identified several major gene classes as candidate essential gene loci for in vivo survival; these include genes for amino acid transporters, oligopeptide transporters, and lantibiotic synthesis (W. R. Schwan, S. N. Coulter, E. Y. W. Ng, M. H. Langhorne, H. D. Ritchie, L. L. Brody, S. Westbrock-Wadman, A. S. Bayer, K. R. Folger, and C. K. Stover, Infect. Immun. 66:567-572, 1998). In this study, we directly compared the virulence of four such isogenic signature tag mutants with that of the parental strain (RN6390) by using a prototypical model of invasive S. aureus infection, experimental endocarditis (IE). The oligonucleotide signature tag (OST) mutant with insertional inactivation of the gene (putP) which encodes the high-affinity transporter for proline uptake exhibited significantly reduced virulence in the IE model across three challenge inocula (10(4) to 10(6) CFU) in terms of achievable intravegetation densities (P, <0.05). The negative impact of putP inactivation on in vivo survival in the IE model was confirmed by simultaneous challenge with the original putP mutant and the parental strain as well as by challenge with a putP mutant in which this genetic inactivation was transduced into a distinct parental strain (S6C). In contrast, inactivation of loci encoding an oligopeptide transporter, a purine repressor, and lantibiotic biosynthesis had no substantial impact on the capacity of OST mutants to survive within IE vegetations. Thus, genes encoding the uptake of essential amino acids may well represent novel targets for new drug development. These data also confirm the utility of the OST technique as an important screening methodology for identifying candidate genes as requisite loci for the in vivo survival of S. aureus.
金黄色葡萄球菌可引发多种侵袭性人类感染。然而,迄今为止尚未明确该病原体在体内存活所必需的基因。先前的研究人员利用特征性标签诱变技术和大型突变体库筛选,确定了几类主要基因作为体内存活的候选必需基因位点;这些基因包括氨基酸转运蛋白、寡肽转运蛋白和羊毛硫抗生素合成相关基因(W. R. 施万、S. N. 库尔特、E. Y. W. 吴、M. H. 兰霍恩、H. D. 里奇、L. L. 布罗迪、S. 韦斯特布罗克 - 瓦德曼、A. S. 拜耳、K. R. 福尔杰和C. K. 斯托弗,《感染与免疫》66:567 - 572,1998年)。在本研究中,我们通过侵袭性金黄色葡萄球菌感染的典型模型——实验性心内膜炎(IE),直接比较了四个此类同基因特征性标签突变体与亲本菌株(RN6390)的毒力。编码脯氨酸高亲和力转运蛋白的基因(putP)发生插入失活的寡核苷酸特征性标签(OST)突变体,在IE模型中,针对三种接种量(10⁴至10⁶CFU),就可达到的赘生物内密度而言,其毒力显著降低(P <0.05)。通过同时用原始putP突变体和亲本菌株进行攻击,以及用将该基因失活转导至不同亲本菌株(S6C)的putP突变体进行攻击,证实了putP失活对IE模型体内存活的负面影响。相比之下,编码寡肽转运蛋白、嘌呤阻遏物和羊毛硫抗生素生物合成的基因座失活,对OST突变体在IE赘生物内存活的能力没有实质性影响。因此,编码必需氨基酸摄取的基因很可能代表了新药开发的新靶点。这些数据也证实了OST技术作为一种重要筛选方法,用于鉴定金黄色葡萄球菌体内存活所需基因位点的候选基因的实用性。