Snow A D, Kinsella M G, Parks E, Sekiguchi R T, Miller J D, Kimata K, Wight T N
Department of Pathology, University of Washington, Seattle 98195-6480, USA.
Arch Biochem Biophys. 1995 Jun 20;320(1):84-95. doi: 10.1006/abbi.1995.1345.
Previous studies have demonstrated the immunolocalization of perlecan, a specific heparan sulfate proteoglycan, to the beta-amyloid protein (A beta)-containing amyloid deposits within the walls of blood vessels (i.e., congophilic angiopathy) in Alzheimer's disease (AD) brain. In the present investigation, the differential binding of previously characterized endothelial cell (EC)- and smooth muscle cell (SMC)-derived PGs to A beta was examined to determine whether the accumulation of A beta in cerebrovascular amyloid deposits may be due to its interactions with perlecan. Pretreatment of AA amyloidotic splenic and liver tissue sections with synthetic A beta (1-28) produced strong immunoreactivity with A beta antibodies at tissue sites enriched in perlecan which was partially removed by pretreatment with heparitinase, but not by chondroitin ABC lyase. [35S]-Sulfate labeled proteoglycans (PGs) derived from cultured ECs and SMCs bound to affinity columns containing A beta (1-28) or (1-40), with virtually no binding to A beta (40-1) (reverse peptide), beta-amyloid precursor protein (410-429), or bovine serum albumin. Characterization of EC and SMC PGs bound to A beta (1-28) revealed strong binding by perlecan, weak binding by decorin and biglycan, two dermatan sulfate proteoglycans, and lack of binding by versican/PG-M, a large chondroitin sulfate proteoglycan. Binding of 125I-labeled perlecan to A beta (1-28) was strongly inhibited by isolated perlecan and to a lesser extent by heparin, but not by chondroitin-6-sulfate or unsulfated dextran sulfate. Heparitinase treatment decreased, but did not eliminate the binding of 125I-labeled perlecan to A beta (1-28). Scatchard analysis of the interaction of A beta (1-28)- and EC-derived perlecan in solid-phase assays indicated high-affinity (Kd = 8.3 x 10(-11) M) and lower-affinity (Kd = 4.2 x 10(-8) M) binding sites, with approximately 1 mol of perlecan binding 1.8 mol of A beta. A significant decrease in binding of EC-derived perlecan to A beta (1-28) was observed when a sequence within the putative heparin-binding motif of A beta (His13His14Gln15Lys16) was replaced by the uncharged peptide sequence, Gly13Gly14Gln15Gly16, indicating a perlecan binding site on A beta near the postulated alpha-secretase site (at Lys-16). Overall, the results indicate that specific vascular cell-derived PGs differentially interact with A beta, and that the interactions of highest affinity occur between A beta and binding sites on both the core protein and glycosaminoglycan chains of perlecan.(ABSTRACT TRUNCATED AT 400 WORDS)
先前的研究已证明,在阿尔茨海默病(AD)脑内,特定的硫酸乙酰肝素蛋白聚糖核心蛋白聚糖(perlecan)免疫定位于血管壁内含有β-淀粉样蛋白(Aβ)的淀粉样沉积物(即嗜刚果红血管病)。在本研究中,检测了先前鉴定的内皮细胞(EC)和平滑肌细胞(SMC)来源的蛋白聚糖(PG)与Aβ的差异结合,以确定脑血管淀粉样沉积物中Aβ的积累是否可能归因于其与核心蛋白聚糖的相互作用。用合成的Aβ(1-28)预处理AA淀粉样变性脾和肝组织切片后,在富含核心蛋白聚糖的组织部位产生了与Aβ抗体的强免疫反应性,用肝素酶预处理可部分去除该反应性,但用软骨素ABC裂解酶预处理则不能。[35S] - 硫酸盐标记的来自培养的EC和SMC的蛋白聚糖与含有Aβ(1-28)或(1-40)的亲和柱结合,几乎不与Aβ(40-1)(反向肽)、β-淀粉样前体蛋白(410-429)或牛血清白蛋白结合。对与Aβ(1-28)结合的EC和SMC PG的表征显示,核心蛋白聚糖有强结合,两种硫酸皮肤素蛋白聚糖饰胶蛋白聚糖和双糖链蛋白聚糖有弱结合,而一种大型硫酸软骨素蛋白聚糖多功能蛋白聚糖/PG-M无结合。125I标记的核心蛋白聚糖与Aβ(1-28)的结合受到分离的核心蛋白聚糖的强烈抑制,肝素在较小程度上也有抑制作用,但硫酸软骨素-6-硫酸盐或未硫酸化的硫酸葡聚糖无此作用。肝素酶处理减少了,但并未消除125I标记的核心蛋白聚糖与Aβ(1-28)的结合。在固相分析中对Aβ(1-28)与EC来源的核心蛋白聚糖相互作用的Scatchard分析表明存在高亲和力(Kd = 8.3×10-11 M)和低亲和力(Kd = 4.2×10-8 M)结合位点,约1摩尔核心蛋白聚糖结合1.8摩尔Aβ。当Aβ假定的肝素结合基序内的序列(His13His14Gln15Lys16)被无电荷肽序列Gly13Gly14Gln15Gly16取代时,观察到EC来源的核心蛋白聚糖与Aβ(1-28)的结合显著减少,这表明Aβ上靠近假定的α-分泌酶位点(在Lys-16处)存在一个核心蛋白聚糖结合位点。总体而言,结果表明特定血管细胞来源的PG与Aβ有差异相互作用,且最高亲和力的相互作用发生在Aβ与核心蛋白聚糖的核心蛋白和糖胺聚糖链上的结合位点之间。(摘要截短于400字)
