Lee Li Ling, Ha HyungHo, Chang Young-Tae, DeLisa Matthew P
Cornell University, Ithaca, New York 14853, USA.
Protein Sci. 2009 Feb;18(2):277-86. doi: 10.1002/pro.33.
Genetic and biochemical studies suggest that Alzheimer's disease (AD) is caused by a series of events initiated by the production and subsequent aggregation of the Alzheimer's amyloid beta peptide (Abeta), the so-called amyloid cascade hypothesis. Thus, a logical approach to treating AD is the development of small molecule inhibitors that either block the proteases that generate Abeta from its precursor (beta- and gamma-secretases) or interrupt and/or reverse Abeta aggregation. To identify potent inhibitors of Abeta aggregation, we have developed a high-throughput screen based on an earlier selection that effectively paired the folding quality control feature of the Escherichia coli Tat protein export system with aggregation of the 42-residue AD pathogenesis effecter Abeta42. Specifically, a tripartite fusion between the Tat-dependent export signal ssTorA, the Abeta42 peptide and the beta-lactamase (Bla) reporter enzyme was found to be export incompetent due to aggregation of the Abeta42 moiety. Here, we reasoned that small, cell-permeable molecules that inhibited Abeta42 aggregation would render the ssTorA-Abeta42-Bla chimera competent for Tat export to the periplasm where Bla is active against beta-lactam antibiotics such as ampicillin. Using a fluorescence-based version of our assay, we screened a library of triazine derivatives and isolated four nontoxic, cell-permeable compounds that promoted efficient Tat-dependent export of ssTorA-Abeta42-Bla. Each of these was subsequently shown to be a bona fide inhibitor of Abeta42 aggregation using a standard thioflavin T fibrillization assay, thereby highlighting the utility of our bacterial assay as a useful screen for antiaggregation factors under physiological conditions.
遗传学和生物化学研究表明,阿尔茨海默病(AD)是由一系列事件引发的,这些事件始于阿尔茨海默病淀粉样β肽(Aβ)的产生及其随后的聚集,即所谓的淀粉样蛋白级联假说。因此,治疗AD的一种合理方法是开发小分子抑制剂,这些抑制剂要么阻断从其前体产生Aβ的蛋白酶(β-和γ-分泌酶),要么中断和/或逆转Aβ聚集。为了鉴定有效的Aβ聚集抑制剂,我们基于早期的筛选方法开发了一种高通量筛选,该筛选有效地将大肠杆菌Tat蛋白输出系统的折叠质量控制特征与42个残基的AD发病效应因子Aβ42的聚集相结合。具体而言,由于Aβ42部分的聚集,发现Tat依赖性输出信号ssTorA、Aβ42肽和β-内酰胺酶(Bla)报告酶之间的三方融合无法输出。在此,我们推断,抑制Aβ42聚集的小的、可透过细胞的分子将使ssTorA-Aβ42-Bla嵌合体能够通过Tat输出到周质,在周质中Bla对氨苄青霉素等β-内酰胺抗生素具有活性。使用我们基于荧光的检测方法,我们筛选了一个三嗪衍生物库,并分离出四种无毒、可透过细胞的化合物,这些化合物促进了ssTorA-Aβ42-Bla的高效Tat依赖性输出。随后,使用标准的硫黄素T纤维化检测方法,证明这些化合物中的每一种都是Aβ42聚集的真正抑制剂,从而突出了我们的细菌检测方法作为在生理条件下筛选抗聚集因子的有用筛选方法的实用性。