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唾液包被的羟基磷灰石表面吸附的葡糖基转移酶的构象和葡聚糖生成的表面诱导变化。

Surface-induced changes in the conformation and glucan production of glucosyltransferase adsorbed on saliva-coated hydroxyapatite.

作者信息

Fears Kenan P, Gonzalez-Begne Mireya, Love Corey T, Day Delbert E, Koo Hyun

机构信息

†Chemistry Division, U.S. Naval Research Laboratory, Washington, D.C. 20375, United States.

‡Department of Dentistry and Center for Oral Biology, University of Rochester Medical Center, Rochester, New York 14642, United States.

出版信息

Langmuir. 2015 Apr 28;31(16):4654-62. doi: 10.1021/la504461h. Epub 2015 Apr 13.

Abstract

Glucosyltransferases (Gtfs) from S. mutans play critical roles in the development of virulent oral biofilms associated with dental caries disease. Gtfs adsorbed to the tooth surface produce glucans that promote local microbial colonization and provide an insoluble exopolysaccharides (EPS) matrix that facilitates biofilm initiation. Moreover, agents that inhibit the enzymatic activity of Gtfs in solution often have reduced or no effects on surface-adsorbed Gtfs. This study elucidated the mechanisms responsible for the differences in functionality that GtfB exhibits in solution vs surface-adsorbed. Upon adsorption to planar fused-quartz substrates, GtfB displayed a 37% loss of helices and 36% increase of β-sheets, as determined by circular dichroism (CD) spectroscopy, and surface-induced conformational changes were more severe on substrates modified with CH3- and NH2-terminated self-assembled monolayers. GtfB also underwent substantial conformation changes when adsorbing to hydroxyapatite (HA) microspheres, likely due to electrostatic interactions between negatively charged GtfB and positively charged HA crystal faces. Conformational changes were lessened when HA surfaces were coated with saliva (sHA) prior to GtfB adsorption. Furthermore, GtfB remained highly active on sHA, as determined by in situ attenuated total reflectance Fourier transform infrared (ATR-FTIR) spectroscopy, producing glucans that were structurally different than GtfB in solution and known to increase the accumulation and virulence of biofilms. Our data provide the first insight into the structural underpinnings governing Gtf conformation and enzymatic function that occur on tooth surfaces in vivo, which may lead to designing potent new inhibitors and improved strategies to combat the formation of pathogenic oral biofilms.

摘要

变形链球菌的葡糖基转移酶(Gtfs)在与龋齿疾病相关的毒性口腔生物膜的形成中起着关键作用。吸附在牙齿表面的Gtfs产生葡聚糖,促进局部微生物定植,并提供一种不溶性胞外多糖(EPS)基质,有助于生物膜的起始。此外,抑制溶液中Gtfs酶活性的试剂通常对表面吸附的Gtfs作用减弱或无效。本研究阐明了GtfB在溶液中与表面吸附时功能差异的机制。通过圆二色性(CD)光谱测定,吸附在平面熔融石英基底上时,GtfB的螺旋结构损失37%,β-折叠增加36%,并且在由甲基和氨基封端的自组装单分子层修饰的基底上,表面诱导的构象变化更严重。当吸附到羟基磷灰石(HA)微球上时,GtfB也发生了显著的构象变化,这可能是由于带负电荷的GtfB与带正电荷的HA晶面之间的静电相互作用。在GtfB吸附之前,当HA表面用唾液(sHA)包被时,构象变化减小。此外,通过原位衰减全反射傅里叶变换红外(ATR-FTIR)光谱测定,GtfB在sHA上仍保持高活性,产生的葡聚糖在结构上不同于溶液中的GtfB,并且已知会增加生物膜的积累和毒性。我们的数据首次深入了解了体内牙齿表面上Gtf构象和酶功能的结构基础,这可能会导致设计出有效的新型抑制剂以及改进对抗致病性口腔生物膜形成的策略。

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