Gomis-Rüth F Xavier, Botelho Tiago O, Bode Wolfram
Proteolysis Lab, Department of Structural Biology, Molecular Biology Institute of Barcelona, CSIC, Barcelona Science Park, Spain.
Biochim Biophys Acta. 2012 Jan;1824(1):157-63. doi: 10.1016/j.bbapap.2011.04.014. Epub 2011 Apr 30.
Visualization of three-dimensional structures is essential to the transmission of information to the general reader and the comparison of related structures. Therefore, it would be useful to provide a common framework. Based on the work of Schechter and Berger, and the finding that most peptidases bind their substrates in extended conformation, we suggest a "standard orientation" for the overall description of metallopeptidases (MPs) as done before for peptidases of other classes. This entails a frontal view of the horizontally-aligned active-site cleft. A substrate is bound N- to C-terminally from left (on the non-primed side of the cleft) to right (on the primed side), and the catalytic metal ion resides at the cleft bottom at roughly half width. This view enables us to see that most metalloendopeptidases are bifurcated into an upper and a lower sub-domain by the cleft, whose back is framed by a nearly horizontal "active-site helix." The latter comprises a short zinc-binding consensus sequence, either HEXXH or HXXEH, which provides two histidines to bind the single catalytic metal and the general-base/acid glutamate required for catalysis. In addition, an oblique "backing helix" is observed behind the active-site helix, and a mixed β-sheet of at least three strands is positioned in the upper sub-domain paralleling the cleft. The lowermost "upper-rim" strand of the sheet runs antiparallel to the substrate bound in the cleft and therefore contributes both to delimitating the cleft top and to binding of the substrate main-chain on its non-primed side through β-ribbon-like interactions. In contrast, in metalloexopeptidases, which chop off N- or C-terminal residues only, extensive binding on both sides of the cleft is not required and a different overall scaffold is generally observed. This consists of an αβα-sandwich, which is reminiscent of, but clearly distinct from, the archetypal α/β-hydrolase fold. Metalloexopeptidases have their active sites at the C-terminal end of a central, eight-stranded twisted β-sheet, and can contain one or two catalytic metal ions. As the zinc-binding site and the residues engaged in substrate binding and catalysis are mainly provided by loops connecting the β-sheet strands and the helices on either side, the respective standard orientations vary with respect to the position of the sheets. The standard orientation of eight prototypic MP structures is presented and discussed. This article is part of a Special Issue entitled: Proteolysis 50 years after the discovery of lysosome.
三维结构的可视化对于向普通读者传递信息以及比较相关结构至关重要。因此,提供一个通用框架会很有用。基于Schechter和Berger的工作,以及大多数肽酶以伸展构象结合其底物这一发现,我们像之前对其他类别的肽酶那样,为金属肽酶(MPs)的整体描述提出一种“标准取向”。这需要对水平排列的活性位点裂隙进行正视图观察。底物从左(在裂隙的非引物侧)到右(在引物侧)以N端到C端的方向结合,催化金属离子位于裂隙底部大约一半宽度处。这种视图使我们能够看到,大多数金属内肽酶被裂隙分为一个上亚结构域和一个下亚结构域,其背面由一个近乎水平的“活性位点螺旋”构成框架。后者包含一个短的锌结合共有序列,即HEXXH或HXXEH,它提供两个组氨酸来结合单个催化金属以及催化所需的通用碱/酸谷氨酸。此外,在活性位点螺旋后方观察到一个倾斜的“支撑螺旋”,并且在与裂隙平行的上亚结构域中定位有至少三条链的混合β折叠。该折叠最下面的“上边缘”链与结合在裂隙中的底物反平行,因此既有助于界定裂隙顶部,又通过类似β带的相互作用在其非引物侧结合底物主链。相比之下,在仅切割N端或C端残基的金属外肽酶中,不需要在裂隙两侧进行广泛结合,并且通常观察到不同的整体支架结构。这由一个αβα三明治组成,它让人联想到但明显不同于典型的α/β水解酶折叠。金属外肽酶的活性位点位于中央八链扭曲β折叠的C端,并且可以包含一个或两个催化金属离子。由于锌结合位点以及参与底物结合和催化的残基主要由连接β折叠链和两侧螺旋的环提供,各自的标准取向相对于折叠的位置会有所不同。本文展示并讨论了八个典型MP结构的标准取向。本文是名为:溶酶体发现50年后的蛋白水解 的特刊的一部分。
