Department of Molecular Biology and Biochemistry, University of California, Irvine, CA 92697, USA.
Mol Neurodegener. 2007 Sep 26;2:18. doi: 10.1186/1750-1326-2-18.
Amyloid-related degenerative diseases are associated with the accumulation of misfolded proteins as amyloid fibrils in tissue. In Alzheimer disease (AD), amyloid accumulates in several distinct types of insoluble plaque deposits, intracellular Abeta and as soluble oligomers and the relationships between these deposits and their pathological significance remains unclear. Conformation dependent antibodies have been reported that specifically recognize distinct assembly states of amyloids, including prefibrillar oligomers and fibrils.
We immunized rabbits with a morphologically homogeneous population of Abeta42 fibrils. The resulting immune serum (OC) specifically recognizes fibrils, but not random coil monomer or prefibrillar oligomers, indicating fibrils display a distinct conformation dependent epitope that is absent in prefibrillar oligomers. The fibril epitope is also displayed by fibrils of other types of amyloids, indicating that the epitope is a generic feature of the polypeptide backbone. The fibril specific antibody also recognizes 100,000 x G soluble fibrillar oligomers ranging in size from dimer to greater than 250 kDa on western blots. The fibrillar oligomers recognized by OC are immunologically distinct from prefibrillar oligomers recognized by A11, even though their sizes overlap broadly, indicating that size is not a reliable indicator of oligomer conformation. The immune response to prefibrillar oligomers and fibrils is not sequence specific and antisera of the same specificity are produced in response to immunization with islet amyloid polypeptide prefibrillar oligomer mimics and fibrils. The fibril specific antibodies stain all types of amyloid deposits in human AD brain. Diffuse amyloid deposits stain intensely with anti-fibril antibody although they are thioflavin S negative, suggesting that they are indeed fibrillar in conformation. OC also stains islet amyloid deposits in transgenic mouse models of type II diabetes, demonstrating its generic specificity for amyloid fibrils.
Since the fibril specific antibodies are conformation dependent, sequence-independent, and recognize epitopes that are distinct from those present in prefibrillar oligomers, they may have broad utility for detecting and characterizing the accumulation of amyloid fibrils and fibrillar type oligomers in degenerative diseases.
淀粉样相关退行性疾病与组织中错误折叠蛋白聚集成淀粉样纤维有关。在阿尔茨海默病(AD)中,淀粉样物质积聚在几种不同类型的不溶性斑块沉积物中,包括细胞内 Abeta 和可溶性寡聚物,这些沉积物及其病理意义之间的关系仍不清楚。已经报道了构象依赖性抗体,它们特异性识别淀粉样物质的不同组装状态,包括前纤维状寡聚物和纤维。
我们用形态均一的 Abeta42 纤维群体免疫兔子。由此产生的免疫血清(OC)特异性识别纤维,但不识别随机卷曲单体或前纤维状寡聚物,表明纤维显示出独特的构象依赖性表位,而前纤维状寡聚物中不存在该表位。该纤维表位也存在于其他类型的淀粉样物质的纤维中,表明该表位是多肽主链的通用特征。纤维特异性抗体也识别大小从二聚体到大于 250 kDa 的 100,000 x G 可溶性纤维状寡聚物。OC 识别的纤维状寡聚物在免疫上与 A11 识别的前纤维状寡聚物不同,尽管它们的大小广泛重叠,表明大小不是寡聚物构象的可靠指标。对前纤维状寡聚物和纤维的免疫反应不是序列特异性的,并且用胰岛淀粉样多肽前纤维状寡聚物模拟物和纤维免疫产生了相同特异性的抗血清。针对前纤维状寡聚物和纤维的免疫反应不是序列特异性的,并且用胰岛淀粉样多肽前纤维状寡聚物模拟物和纤维免疫产生了相同特异性的抗血清。纤维特异性抗体可染色人类 AD 大脑中所有类型的淀粉样沉积物。弥漫性淀粉样沉积物用抗纤维抗体强烈染色,尽管它们对硫黄素 S 呈阴性,这表明它们在构象上确实是纤维状的。OC 还染色转染小鼠模型中的胰岛淀粉样沉积物,证明其对淀粉样纤维的通用特异性。
由于纤维特异性抗体是构象依赖性的、序列非依赖性的,并且识别的表位与前纤维状寡聚物中的表位不同,因此它们可能具有广泛的用途,用于检测和表征退行性疾病中淀粉样纤维和纤维状寡聚物的积累。
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