Division of Immunology and Molecular Medicine, Okinaka Memorial Institute for Medical Research, Tokyo, Japan.
Department of Endocrinology and Metabolism, Toranomon Hospital, Tokyo, Japan.
J Diabetes Investig. 2022 Mar;13(3):435-442. doi: 10.1111/jdi.13700. Epub 2021 Dec 8.
AIMS/INTRODUCTION: The need for antiserum for immunohistochemical (IHC) detection of enterovirus (EV) in formaldehyde-fixed and paraffin-embedded samples is increasing. The gold standard monoclonal antibody (clone 5D8/1) against EV-envelope protein (VP1) was proven to cross-react with other proteins. Another candidate marker of EV proteins is 2A protease (2A ), which is encoded by the EV gene and translated by the host cells during EV replication, and participates processing proproteins to viral capsid proteins.
We raised polyclonal antiserum by immunizing a rabbit with an 18-mer peptide of Coxsackievirus B1 (CVB1)-2A , and examined the specificity and sensitivity for EV on formaldehyde-fixed and paraffin-embedded tissue samples.
Enzyme-linked immunosorbent assay study showed a high titer of antibody for 18-mer peptide of CVB1-2A , cross-reacting with CVB3-2A peptide. IHC showed that antiserum against 2A reacted with CVB1-infected and VP1-positive Vero cells. Confocal laser scanning microscopy showed that antigen stained by the 2A antibody located in the same cell with VP1 stained by 5D8/1. IHC using 2A antiserum showed dense staining in the islets of EV-associated fulminant type 1 diabetes pancreas and that located in the same cell stained positive for VP1 (5D8/1). Specificity of 2A antiserum by IHC staining was confirmed by negative 2A in 14 VP1-negative non-diabetes control pancreases.
Our study provides a new polyclonal antiserum against CVB1-2A , which might be useful for IHC of EV-infected human tissues stored as archive of formaldehyde-fixed and paraffin-embedded tissue samples.
目的/引言:在甲醛固定和石蜡包埋样本中进行肠病毒(EV)免疫组织化学(IHC)检测时,对抗血清的需求不断增加。针对 EV 包膜蛋白(VP1)的金标准单克隆抗体(克隆 5D8/1)已被证明会与其他蛋白发生交叉反应。EV 蛋白的另一个候选标志物是 2A 蛋白酶(2A),它由 EV 基因编码,并在 EV 复制过程中由宿主细胞翻译,参与将前蛋白加工成病毒衣壳蛋白。
我们通过用 Coxsackievirus B1(CVB1)-2A 的 18 肽免疫兔子来制备多克隆抗血清,并在甲醛固定和石蜡包埋组织样本中检测其对 EV 的特异性和敏感性。
酶联免疫吸附试验研究显示,针对 CVB1-2A 18 肽的抗体效价很高,与 CVB3-2A 肽发生交叉反应。IHC 显示,针对 2A 的抗血清与感染 CVB1 且 VP1 阳性的 Vero 细胞反应。共聚焦激光扫描显微镜显示,2A 抗体染色的抗原与 5D8/1 染色的 VP1 位于同一细胞内。使用 2A 抗血清进行 IHC 显示,在与 EV 相关的暴发性 1 型糖尿病胰腺的胰岛中存在密集染色,且与 VP1(5D8/1)染色阳性的细胞位于同一细胞内。通过 IHC 染色对 2A 抗血清的特异性进行了确认,在 14 例 VP1 阴性的非糖尿病对照胰腺中,2A 均呈阴性。
本研究提供了针对 CVB1-2A 的新型多克隆抗血清,可能对保存于甲醛固定和石蜡包埋组织样本档案中的 EV 感染人类组织的 IHC 有用。
