Institute for Regenerative Medicine, University of Zurich, 8952, Schlieren, Switzerland.
Present Address: Department of Chemistry University of Cologne, Institute of Biochemistry, 50674, Cologne, Germany.
Acta Neuropathol Commun. 2019 Dec 3;7(1):194. doi: 10.1186/s40478-019-0846-8.
An impairment of amyloid β-peptide (Aβ) clearance is suggested to play a key role in the pathogenesis of sporadic Alzheimer's disease (AD). Amyloid degradation is mediated by various mechanisms including fragmentation by enzymes like neprilysin, matrix metalloproteinases (MMPs) and a recently identified amyloidolytic activity of β-site amyloid precursor protein cleaving enzyme 1 (BACE1). BACE1 cleavage of Aβ40 and Aβ42 results in the formation of a common Aβ34 intermediate which was found elevated in cerebrospinal fluid levels of patients at the earliest disease stages. To further investigate the role of Aβ34 as a marker for amyloid clearance in AD, we performed a systematic and comprehensive analysis of Aβ34 immunoreactivity in hippocampal and cortical post-mortem brain tissue from AD patients and non-demented elderly individuals. In early Braak stages, Aβ34 was predominantly detectable in a subset of brain capillaries associated with pericytes, while in later disease stages, in clinically diagnosed AD, this pericyte-associated Aβ34 immunoreactivity was largely lost. Aβ34 was also detected in isolated human cortical microvessels associated with brain pericytes and its levels correlated with Aβ40, but not with Aβ42 levels. Moreover, a significantly decreased Aβ34/Aβ40 ratio was observed in microvessels from AD patients in comparison to non-demented controls suggesting a reduced proteolytic degradation of Aβ40 to Aβ34 in AD. In line with the hypothesis that pericytes at the neurovascular unit are major producers of Aβ34, biochemical studies in cultured human primary pericytes revealed a time and dose dependent increase of Aβ34 levels upon treatment with recombinant Aβ40 peptides while Aβ34 production was impaired when Aβ40 uptake was reduced or BACE1 activity was inhibited. Collectively, our findings indicate that Aβ34 is generated by a novel BACE1-mediated Aβ clearance pathway in pericytes of brain capillaries. As amyloid clearance is significantly reduced in AD, impairment of this pathway might be a major driver of the pathogenesis in sporadic AD.
淀粉样β肽(Aβ)清除能力的损害被认为在散发性阿尔茨海默病(AD)的发病机制中起关键作用。淀粉样蛋白的降解是通过多种机制介导的,包括酶如 Neprilysin、基质金属蛋白酶(MMPs)和最近发现的β-位点淀粉样前体蛋白裂解酶 1(BACE1)的淀粉样蛋白水解活性的片段化。BACE1 对 Aβ40 和 Aβ42 的切割导致形成一种常见的 Aβ34 中间产物,在疾病早期阶段患者的脑脊液水平中发现该中间产物升高。为了进一步研究 Aβ34 作为 AD 中淀粉样蛋白清除的标志物的作用,我们对 AD 患者和非痴呆老年人的海马和皮质死后脑组织中的 Aβ34 免疫反应进行了系统和全面的分析。在早期 Braak 阶段,Aβ34 主要在与周细胞相关的一组脑毛细血管中可检测到,而在晚期疾病阶段,即临床上诊断为 AD 时,这种与周细胞相关的 Aβ34 免疫反应大部分丢失。Aβ34 也在与脑周细胞相关的分离的人皮质微血管中被检测到,其水平与 Aβ40 相关,但与 Aβ42 水平不相关。此外,与非痴呆对照组相比,AD 患者的微血管中 Aβ34/Aβ40 比值显著降低,提示 AD 中 Aβ40 向 Aβ34 的蛋白水解降解减少。与周细胞在神经血管单元中是 Aβ34 的主要产生者的假说一致,在培养的人原代周细胞中的生化研究表明,在用重组 Aβ40 肽处理时,Aβ34 水平随时间和剂量依赖性增加,而当 Aβ40 摄取减少或 BACE1 活性被抑制时,Aβ34 的产生受损。总的来说,我们的研究结果表明,Aβ34 是由脑毛细血管周细胞中一种新的 BACE1 介导的 Aβ 清除途径产生的。由于 AD 中淀粉样蛋白清除明显减少,这种途径的损伤可能是散发性 AD 发病机制的主要驱动因素。
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