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小短乳杆菌表面层在脂质体上重新组装后的结构与天然结构不同,这一点由小角X射线散射(SAXS)揭示。

The structure of Lactobacillus brevis surface layer reassembled on liposomes differs from native structure as revealed by SAXS.

作者信息

Kontro Inkeri, Wiedmer Susanne K, Hynönen Ulla, Penttilä Paavo A, Palva Airi, Serimaa Ritva

机构信息

Department of Physics, P.O.B. 64, 00014 University of Helsinki, Finland.

Department of Chemistry, P.O.B. 55, 00014 University of Helsinki, Finland.

出版信息

Biochim Biophys Acta. 2014 Aug;1838(8):2099-104. doi: 10.1016/j.bbamem.2014.04.022. Epub 2014 May 4.

DOI:10.1016/j.bbamem.2014.04.022
PMID:24796504
Abstract

The reassembly of the S-layer protein SlpA of Lactobacillus brevis ATCC 8287 on positively charged liposomes was studied by small angle X-ray scattering (SAXS) and zeta potential measurements. SlpA was reassembled on unilamellar liposomes consisting of 1-palmitoyl-2-oleyl-sn-glycero-3-phosphocholine and 1,2-dioleoyl-3-trimethylammonium-propane, prepared by extrusion through membranes with pore sizes of 50nm and 100nm. Similarly extruded samples without SlpA were used as a reference. The SlpA-containing samples showed clear diffraction peaks in their SAXS intensities. The lattice constants were calculated from the diffraction pattern and compared to those determined for SlpA on native cell wall fragments. Lattice constants for SlpA reassembled on liposomes (a=9.29nm, b=8.03nm, and γ=84.9°) showed a marked change in the lattice constants b and γ when compared to those determined for SlpA on native cell wall fragments (a=9.41nm, b=6.48nm, and γ=77.0°). The latter are in good agreement with values previously determined by electron microscopy. This indicates that the structure formed by SlpA is stable on the bacterial cell wall, but SlpA reassembles into a different structure on cationic liposomes. From the (10) reflection, the lower limit of crystallite size of SlpA on liposomes was determined to be 92nm, corresponding to approximately ten aligned lattice planes.

摘要

通过小角X射线散射(SAXS)和zeta电位测量研究了短乳杆菌ATCC 8287的S层蛋白SlpA在带正电荷脂质体上的重新组装。SlpA在由1-棕榈酰-2-油酰-sn-甘油-3-磷酸胆碱和1,2-二油酰-3-三甲基铵丙烷组成的单层脂质体上重新组装,这些脂质体通过孔径为50nm和100nm的膜挤压制备。将不含SlpA的类似挤压样品用作参考。含SlpA的样品在其SAXS强度中显示出清晰的衍射峰。从衍射图谱计算晶格常数,并与在天然细胞壁片段上测定的SlpA的晶格常数进行比较。与在天然细胞壁片段上测定的SlpA的晶格常数(a = 9.41nm,b = 6.48nm,γ = 77.0°)相比,在脂质体上重新组装的SlpA的晶格常数(a = 9.29nm,b = 8.03nm,γ = 84.9°)显示出晶格常数b和γ的显著变化。后者与先前通过电子显微镜测定的值非常吻合。这表明由SlpA形成的结构在细菌细胞壁上是稳定的,但SlpA在阳离子脂质体上重新组装成不同的结构。根据(10)反射,确定脂质体上SlpA微晶尺寸的下限为9

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