准确评估程序性死亡配体1需要在循环肿瘤细胞识别中具有高特异性。
High Specificity in Circulating Tumor Cell Identification Is Required for Accurate Evaluation of Programmed Death-Ligand 1.
作者信息
Schehr Jennifer L, Schultz Zachery D, Warrick Jay W, Guckenberger David J, Pezzi Hannah M, Sperger Jamie M, Heninger Erika, Saeed Anwaar, Leal Ticiana, Mattox Kara, Traynor Anne M, Campbell Toby C, Berry Scott M, Beebe David J, Lang Joshua M
机构信息
Carbone Cancer Center, University of Wisconsin-Madison, Madison, Wisconsin, United States of America.
Department of Biomedical Engineering, University of Wisconsin-Madison, Madison, Wisconsin, United States of America.
出版信息
PLoS One. 2016 Jul 26;11(7):e0159397. doi: 10.1371/journal.pone.0159397. eCollection 2016.
BACKGROUND
Expression of programmed-death ligand 1 (PD-L1) in non-small cell lung cancer (NSCLC) is typically evaluated through invasive biopsies; however, recent advances in the identification of circulating tumor cells (CTCs) may be a less invasive method to assay tumor cells for these purposes. These liquid biopsies rely on accurate identification of CTCs from the diverse populations in the blood, where some tumor cells share characteristics with normal blood cells. While many blood cells can be excluded by their high expression of CD45, neutrophils and other immature myeloid subsets have low to absent expression of CD45 and also express PD-L1. Furthermore, cytokeratin is typically used to identify CTCs, but neutrophils may stain non-specifically for intracellular antibodies, including cytokeratin, thus preventing accurate evaluation of PD-L1 expression on tumor cells. This holds even greater significance when evaluating PD-L1 in epithelial cell adhesion molecule (EpCAM) positive and EpCAM negative CTCs (as in epithelial-mesenchymal transition (EMT)).
METHODS
To evaluate the impact of CTC misidentification on PD-L1 evaluation, we utilized CD11b to identify myeloid cells. CTCs were isolated from patients with metastatic NSCLC using EpCAM, MUC1 or Vimentin capture antibodies and exclusion-based sample preparation (ESP) technology.
RESULTS
Large populations of CD11b+CD45lo cells were identified in buffy coats and stained non-specifically for intracellular antibodies including cytokeratin. The amount of CD11b+ cells misidentified as CTCs varied among patients; accounting for 33-100% of traditionally identified CTCs. Cells captured with vimentin had a higher frequency of CD11b+ cells at 41%, compared to 20% and 18% with MUC1 or EpCAM, respectively. Cells misidentified as CTCs ultimately skewed PD-L1 expression to varying degrees across patient samples.
CONCLUSIONS
Interfering myeloid populations can be differentiated from true CTCs with additional staining criteria, thus improving the specificity of CTC identification and the accuracy of biomarker evaluation.
背景
非小细胞肺癌(NSCLC)中程序性死亡配体1(PD-L1)的表达通常通过侵入性活检来评估;然而,循环肿瘤细胞(CTC)鉴定方面的最新进展可能是一种侵入性较小的用于此目的的肿瘤细胞检测方法。这些液体活检依赖于从血液中的不同细胞群体中准确鉴定CTC,其中一些肿瘤细胞与正常血细胞具有共同特征。虽然许多血细胞因其高表达CD45而可被排除,但中性粒细胞和其他未成熟髓系亚群的CD45表达低或无表达,并且也表达PD-L1。此外,细胞角蛋白通常用于鉴定CTC,但中性粒细胞可能会对包括细胞角蛋白在内的细胞内抗体进行非特异性染色,从而妨碍对肿瘤细胞上PD-L1表达的准确评估。在评估上皮细胞粘附分子(EpCAM)阳性和EpCAM阴性CTC中的PD-L1时(如在上皮-间质转化(EMT)中),这一点尤为重要。
方法
为了评估CTC误识别对PD-L1评估的影响,我们利用CD11b来鉴定髓系细胞。使用EpCAM、MM黏黏蛋白1(MUC1)或波形蛋白捕获抗体以及基于排除的样本制备(ESP)技术,从转移性NSCLC患者中分离出CTC。
结果
在血沉棕黄层中鉴定出大量CD11b + CD45lo细胞,它们对包括细胞角蛋白在内的细胞内抗体进行非特异性染色。误识别为CTC的CD11b +细胞数量在患者之间有所不同;占传统鉴定的CTC的33% - 100%。用波形蛋白捕获的细胞中CD11b +细胞的频率更高,为41%,而用MUC1或EpCAM捕获的细胞中该频率分别为20%和18%。误识别为CTC的细胞最终在不同患者样本中不同程度地扭曲了PD-L1表达。
结论
通过额外的染色标准,可以将干扰性髓系群体与真正的CTC区分开来,从而提高CTC鉴定的特异性和生物标志物评估的准确性。
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