Department of Physiology, School of Medicine, National and Kapodistrian University of Athens, Athens, Greece.
Division of Immunology and Rheumatology, Hannover Medical University, Hannover, Germany.
Front Immunol. 2021 Jun 18;12:683623. doi: 10.3389/fimmu.2021.683623. eCollection 2021.
B-cell non-Hodgkin's lymphoma (B-NHL) is one of the major complications of primary Sjögren's syndrome (SS). Chronic inflammation and macrophages in SS minor salivary glands have been previously suggested as significant predictors for lymphoma development among SS patients. Lipoprotein-associated phospholipase A2 (Lp-PLA2)-a product mainly of tissue macrophages-is found in the circulation associated with lipoproteins and has been previously involved in cardiovascular, autoimmune, and malignant diseases, including lymphoma.
The purpose of the current study was to investigate the contributory role of Lp-PLA2 in B-NHL development in the setting of primary SS.
Lp-PLA2 activity in serum samples collected from 50 primary SS patients with no lymphoma (SS-nL), 9 primary SS patients with lymphoma (SS-L), and 42 healthy controls (HC) was determined by detection of [H]PAF degradation products by liquid scintillation counter. Moreover, additional sera from 50 SS-nL, 28 SS-L, and 32 HC were tested for Lp-PLA2 activity using a commercially available ELISA kit. Lp-PLA2 mRNA, and protein expression in minor salivary gland (MSG) tissue samples derived from SS-nL, SS-L patients, and sicca controls (SC) were analyzed by real-time PCR, Western blot, and immunohistochemistry.
Serum Lp-PLA2 activity was significantly increased in SS-L compared to both SS-nL and HC by two independent methods implemented [mean ± SD (nmol/min/ml): 62.0 ± 13.4 47.6 ± 14.4 50.7 ± 16.6, p-values: 0.003 and 0.04, respectively, and 19.4 ± 4.5 15.2 ± 3.3 14.5 ± 3.0, p-values: <0.0001, in both comparisons]. ROC analysis revealed that the serum Lp-PLA2 activity measured either by radioimmunoassay or ELISA has the potential to distinguish between SS-L and SS-nL patients (area under the curve [AUC]: 0.8022, CI [95%]: 0.64-0.96, p-value: 0.004 for radioimmunoassay, and AUC: 0.7696, CI [95%]: 0.66-0.88, p-value: <0.0001, for ELISA). Lp-PLA2 expression in MSG tissues was also increased in SS-L compared to SS-nL and SC at both mRNA and protein level. ROC analysis revealed that both MSG mRNA and protein Lp-PLA2 have the potential to distinguish between SS-nL and SS-L patients (area under the curve [AUC] values of 0.8490, CI [95%]: 0.71-0.99, p-value: 0.0019 and 0.9444, CI [95%]: 0.79-1.00, p- value: 0.0389 respectively). No significant difference in either serum Lp-PLA2 activity or MSG tissue expression was observed between SS-nL and HC.
Lp-PLA2 serum activity and MSG tissue mRNA/protein expression could be a new biomarker and possibly a novel therapeutic target for B-cell lymphoproliferation in the setting of SS.
B 细胞非霍奇金淋巴瘤(B-NHL)是原发性干燥综合征(SS)的主要并发症之一。先前有研究表明,SS 患者小唾液腺中的慢性炎症和巨噬细胞是淋巴瘤发展的重要预测因子。脂蛋白相关磷脂酶 A2(Lp-PLA2)-主要来源于组织巨噬细胞-与脂蛋白结合存在于循环中,先前与心血管疾病、自身免疫性疾病和恶性疾病(包括淋巴瘤)有关。
本研究旨在探讨 Lp-PLA2 在原发性 SS 中 B-NHL 发展中的作用。
通过液体闪烁计数器检测 [H]PAF 降解产物,检测 50 例无淋巴瘤原发性 SS 患者(SS-nL)、9 例原发性 SS 合并淋巴瘤患者(SS-L)和 42 例健康对照者(HC)血清样本中的 Lp-PLA2 活性。此外,还使用商业 ELISA 试剂盒检测了另外 50 例 SS-nL、28 例 SS-L 和 32 例 HC 的血清 Lp-PLA2 活性。通过实时 PCR、Western blot 和免疫组化分析 SS-nL、SS-L 患者和干燥综合征对照者(SC)小唾液腺(MSG)组织样本中的 Lp-PLA2 mRNA 和蛋白表达。
两种独立方法检测到,SS-L 患者的血清 Lp-PLA2 活性明显高于 SS-nL 和 HC[平均±标准差(nmol/min/ml):62.0±13.4 47.6±14.4 50.7±16.6,p 值:0.003 和 0.04,分别,和 19.4±4.5 15.2±3.3 14.5±3.0,p 值:<0.0001,在两种比较中]。ROC 分析显示,通过放射免疫分析或 ELISA 测量的血清 Lp-PLA2 活性有可能区分 SS-L 和 SS-nL 患者(曲线下面积 [AUC]:0.8022,CI [95%]:0.64-0.96,p 值:0.004 放射免疫分析,和 AUC:0.7696,CI [95%]:0.66-0.88,p 值:<0.0001,用于 ELISA)。SS-L 患者的 MSG 组织中 Lp-PLA2 表达在 mRNA 和蛋白水平上也高于 SS-nL 和 SC。ROC 分析显示,MSG 组织中的 mRNA 和蛋白 Lp-PLA2 均有可能区分 SS-nL 和 SS-L 患者(AUC 值分别为 0.8490、CI [95%]:0.71-0.99、p 值:0.0019 和 0.9444、CI [95%]:0.79-1.00、p 值:0.0389)。SS-nL 和 HC 之间的血清 Lp-PLA2 活性或 MSG 组织表达无显著差异。
Lp-PLA2 血清活性和 MSG 组织 mRNA/蛋白表达可能是 SS 中 B 细胞淋巴增生的新生物标志物和潜在治疗靶点。
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