Abdul Halim Mohd Farid, Karch Kelly R, Zhou Yitian, Haft Daniel H, Garcia Benjamin A, Pohlschroder Mechthild
University of Pennsylvania, Department of Biology, Philadelphia, Pennsylvania, USA.
University of Pennsylvania, Perelman School of Medicine, Department of Biochemistry and Molecular Biophysics, Penn Medicine Epigenetics Program, Philadelphia, Pennsylvania, USA.
J Bacteriol. 2015 Dec 28;198(5):808-15. doi: 10.1128/JB.00849-15.
For years, the S-layer glycoprotein (SLG), the sole component of many archaeal cell walls, was thought to be anchored to the cell surface by a C-terminal transmembrane segment. Recently, however, we demonstrated that the Haloferax volcanii SLG C terminus is removed by an archaeosortase (ArtA), a novel peptidase. SLG, which was previously shown to be lipid modified, contains a C-terminal tripartite structure, including a highly conserved proline-glycine-phenylalanine (PGF) motif. Here, we demonstrate that ArtA does not process an SLG variant where the PGF motif is replaced with a PFG motif (slg(G796F,F797G)). Furthermore, using radiolabeling, we show that SLG lipid modification requires the PGF motif and is ArtA dependent, lending confirmation to the use of a novel C-terminal lipid-mediated protein-anchoring mechanism by prokaryotes. Similar to the case for the ΔartA strain, the growth, cellular morphology, and cell wall of the slg(G796F,F797G) strain, in which modifications of additional H. volcanii ArtA substrates should not be altered, are adversely affected, demonstrating the importance of these posttranslational SLG modifications. Our data suggest that ArtA is either directly or indirectly involved in a novel proteolysis-coupled, covalent lipid-mediated anchoring mechanism. Given that archaeosortase homologs are encoded by a broad range of prokaryotes, it is likely that this anchoring mechanism is widely conserved.
Prokaryotic proteins bound to cell surfaces through intercalation, covalent attachment, or protein-protein interactions play critical roles in essential cellular processes. Unfortunately, the molecular mechanisms that anchor proteins to archaeal cell surfaces remain poorly characterized. Here, using the archaeon H. volcanii as a model system, we report the first in vivo studies of a novel protein-anchoring pathway involving lipid modification of a peptidase-processed C terminus. Our findings not only yield important insights into poorly understood aspects of archaeal biology but also have important implications for key bacterial species, including those of the human microbiome. Additionally, insights may facilitate industrial applications, given that photosynthetic cyanobacteria encode uncharacterized homologs of this evolutionarily conserved enzyme, or may spur development of unique drug delivery systems.
多年来,许多古细菌细胞壁的唯一成分S层糖蛋白(SLG)被认为通过C端跨膜片段锚定在细胞表面。然而,最近我们证明嗜盐栖热菌的SLG C端被一种新型肽酶——古分选酶(ArtA)切除。SLG此前已被证明发生了脂质修饰,它含有一个C端三联结构,包括一个高度保守的脯氨酸 - 甘氨酸 - 苯丙氨酸(PGF)基序。在此,我们证明ArtA不会处理PGF基序被PFG基序取代的SLG变体(slg(G796F,F797G))。此外,通过放射性标记,我们表明SLG脂质修饰需要PGF基序且依赖于ArtA,这证实了原核生物使用一种新型的C端脂质介导的蛋白质锚定机制。与ΔartA菌株的情况类似,slg(G796F,F797G)菌株的生长、细胞形态和细胞壁受到不利影响,在该菌株中嗜盐栖热菌其他ArtA底物的修饰不应改变,这证明了这些翻译后SLG修饰的重要性。我们的数据表明ArtA直接或间接参与了一种新型的蛋白水解偶联的共价脂质介导的锚定机制。鉴于广泛的原核生物都编码古分选酶同源物,这种锚定机制可能广泛保守。
通过插入、共价连接或蛋白质 - 蛋白质相互作用与细胞表面结合的原核生物蛋白质在基本细胞过程中起关键作用。不幸的是,将蛋白质锚定到古细菌细胞表面的分子机制仍未得到充分表征。在此,我们以嗜盐栖热菌古菌作为模型系统,首次报道了涉及肽酶处理的C端脂质修饰的新型蛋白质锚定途径的体内研究。我们的发现不仅为了解甚少的古细菌生物学方面提供了重要见解,而且对关键细菌物种,包括人类微生物组中的细菌物种也有重要意义。此外,鉴于光合蓝细菌编码这种进化上保守酶的未表征同源物,这些见解可能有助于工业应用,或者可能推动独特药物递送系统的开发。
