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一种标记有链霉亲和素结合肽的纳米抗体的开发及其在血清甲胎蛋白的Luminex荧光免疫分析中的应用。

Development of a nanobody tagged with streptavidin-binding peptide and its application in a Luminex fluoroimmunoassay for alpha fetal protein in serum.

作者信息

Chen Qi, Sun Danyang, Pei Hua, Su Benchao, Bao Kunlu, Cao Hongmei, Zhang Chenghui, Hammock Bruce D, Liu Xing

机构信息

College of Food Science and Engineering, Hainan University Haikou 570228 China

Department of Clinical Laboratory, The Second Affiliated Hospital of Hainan Medical University Haikou 570311 China

出版信息

RSC Adv. 2020 Jun 22;10(40):23767-23774. doi: 10.1039/d0ra04210b. eCollection 2020 Jun 19.

Abstract

Sensitive and accurate detection of disease-related biomarkers can promote the early screening and diagnosis of cancers for improving the prognosis and survival of patients. Herein alpha fetal protein (AFP) was selected as the model macromolecule antigen and we developed AFP-specific alpaca nanobodies (Nbs) from an immunized phage-displayed Nb library. Then Nbs tagged with streptavidin-binding peptide (Nb-SBP) were constructed and used to develop an Nb-SBP-mediated fluoroimmunoassay based on the Luminex-200 system (NS-LFIA). Based on the optimal experimental conditions, the NS-LFIA has a limit of detection of 0.237 ng mL with a linear detection range of 0.49-125 ng mL. The average recovery rate and relative standard derivation were in the range of 98.2-110% and 2.8-13.8%, respectively. The NS-LFIA is highly selective for AFP and ignorable cross-reaction was observed with the other biomarkers. The content of AFP in clinical serum samples was determined by both the developed NS-LFIA and the Roche E601 automatic chemiluminescence immunoassay analyzer and a good correlation was obtained between the two methods ( = 0.9894). Moreover, the Nb-SBP can significantly improve the homogeneity of the fluorescent signals tested by the Luminex-200 system compared with the biotinylated conventional monoclonal antibodies, which could reduce the magnetic microsphere consumption and test cost by decreasing the repetitions of each sample. Thus the results demonstrated that the Nb-SBP was a very promising immunological diagnostic reagent and indicated the applicability and reliability of the NS-LFIA for sensitive detection of AFP and other disease-related biomarkers.

摘要

对疾病相关生物标志物进行灵敏且准确的检测,可促进癌症的早期筛查与诊断,从而改善患者的预后及生存率。在此,选择甲胎蛋白(AFP)作为模型大分子抗原,并从免疫的噬菌体展示纳米抗体(Nb)文库中开发出AFP特异性羊驼纳米抗体。随后构建了标记有链霉亲和素结合肽的纳米抗体(Nb-SBP),并用于开发基于Luminex-200系统的Nb-SBP介导的荧光免疫分析方法(NS-LFIA)。基于最佳实验条件,NS-LFIA的检测限为0.237 ng/mL,线性检测范围为0.49 - 125 ng/mL。平均回收率和相对标准偏差分别在98.2% - 110%和2.8% - 13.8%范围内。NS-LFIA对AFP具有高度选择性,与其他生物标志物的交叉反应可忽略不计。通过所开发的NS-LFIA和罗氏E601自动化学发光免疫分析仪测定临床血清样本中AFP的含量,两种方法之间具有良好的相关性(r = 0.9894)。此外,与生物素化的传统单克隆抗体相比,Nb-SBP可显著提高Luminex-200系统检测的荧光信号的均匀性,这可通过减少每个样本的重复次数来降低磁微球消耗和检测成本。因此,结果表明Nb-SBP是一种非常有前景的免疫诊断试剂,并表明NS-LFIA用于灵敏检测AFP和其他疾病相关生物标志物的适用性和可靠性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/98dd/9054930/8140bdc6109e/d0ra04210b-f1.jpg

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