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肝癌中免疫细胞和生物标志物变化的临床意义

Clinical significance of immune cell and biomarker changes in liver cancer.

作者信息

Zhou Su-Tao, Zhang Bin, Ma Ke, Guo Juan

机构信息

Department of Laboratory Medicine, The First Affiliated Hospital of Hebei North University, Zhangjiakou 075000, Hebei Province, China.

出版信息

World J Gastrointest Surg. 2025 Jun 27;17(6):104923. doi: 10.4240/wjgs.v17.i6.104923.

DOI:10.4240/wjgs.v17.i6.104923
PMID:40584484
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12188603/
Abstract

BACKGROUND

Primary liver cancer (PLC) is characterized by high malignancy, rapid disease progression, and persistent high incidence and mortality rates, posing a significant public health challenge worldwide. Early diagnosis and assessment of PLC are of great significance for guiding clinical treatment and improving patient prognosis. Alpha fetoprotein (AFP) and gamma-glutamyl transpeptidase (GGT) are commonly utilized tumor markers for the clinical diagnosis of PLC. They are ideal indicators for the detection of metastasis and recurrence after LC surgery. Nevertheless, not all patients with PLC secrete large amounts of AFP and GGT, which affects the accuracy of evaluating PLC by monitoring these two tumor markers alone. Cluster of differentiation 3 and 161 double-positive natural killer T (CD3CD161NKT) cell subsets are a class of molecules inextricably related to immune function and tumor occurrence and development. This research seeks to explore the clinical significance of CD3CD161NKT cell subsets combined with tumor markers AFP and GGT in the diagnosis of patients with PLC.

AIM

To probe the clinical significance of CD3CD161NKT cell subsets and AFP and GGT changes in the peripheral blood of individuals with PLC.

METHODS

The PLC group comprised 30 patients diagnosed with PLC who were admitted to our hospital between July 2022 and December 2023, whereas the control group consisted of 30 healthy individuals undergoing routine physical examinations at our hospital. Peripheral blood samples were harvested from both cohorts of patients. The levels of CD4NKT, CD8NKT, CD3CD56NKT, CD8CD56NKT, CD3CD161NKT, and CD3CD161NKT were measured by flow cytometry. Serum AFP content was determined using a fully automatic immunoassay analyzer, and serum GGT content was ascertained by a fully automatic biochemical analyzer. The diagnostic value of CD3CD161NKT cell subsets and AFP and GGT level alterations for PLC was evaluated by receiver operating characteristic curve analysis.

RESULTS

No significant disparities were observed in the counts of white blood cells, neutrophils, and platelets, as well as the levels of blood urea nitrogen and serum creatinine between the two groups ( > 0.05). Lymphocytes, red blood cells, hemoglobin, total protein, albumin, and globulin were more attenuated in the PLC group than in the control group, while glutamic-pyruvic transaminase, glutamic oxalacetic transaminase, and carcinoembryonic antigen levels were increased in the PLC cohort compared with the control cohort, with statistical significance ( < 0.05). No substantial difference was discovered in peripheral blood CD4NKT, CD8NKT, and CD3CD56NKT cells between the two cohorts ( > 0.05). The percentage of CD8CD56NKT cells (8.35% ± 1.01%), CD3CD161NKT cells (14.36% ± 1.55%), and CD3CD161NKT cells (12.08% ± 1.34%) in the PLC group was higher than that in the control group ( < 0.05). The levels of AFP (335.71 ± 20.89 ng/mL) and GGT (136.87 ± 15.62 U/mL) in the PLC cohort were elevated within the PLC cohort compared with the control cohort ( < 0.05). The sensitivity of CD8CD56NKT, CD3CD161NKT, CD3CD161NKT, AFP, and GGT alone for diagnosing PLC was 70.00%, 83.33%, 80.00%, 56.67%, and 53.33%, respectively ( < 0.05), with specificity rates of 66.67%, 80.00%, 76.67%, 76.67%, and 66.67%, respectively ( < 0.05). The area under the curve for combined detection was 0.898, with a sensitivity of 86.67% and a specificity of 80.00% ( < 0.05).

CONCLUSION

The levels of CD8CD56NKT, CD3CD161NKT, CD3CD161NKT, AFP, and GGT in the peripheral blood of patients with PLC were markedly elevated. The combined detection of these five indicators can improve the sensitivity and specificity of PLC diagnosis, providing solid evidence for the early clinical diagnosis of PLC.

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d592/12188603/fdeaf10aefd2/wjgs-17-6-104923-g002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d592/12188603/eb10dc7ba77c/wjgs-17-6-104923-g001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d592/12188603/fdeaf10aefd2/wjgs-17-6-104923-g002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d592/12188603/eb10dc7ba77c/wjgs-17-6-104923-g001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d592/12188603/fdeaf10aefd2/wjgs-17-6-104923-g002.jpg
摘要

背景

原发性肝癌(PLC)具有高恶性、疾病进展迅速以及发病率和死亡率持续居高不下的特点,在全球范围内构成了重大的公共卫生挑战。PLC的早期诊断和评估对于指导临床治疗及改善患者预后具有重要意义。甲胎蛋白(AFP)和γ-谷氨酰转肽酶(GGT)是临床诊断PLC常用的肿瘤标志物。它们是肝癌手术后检测转移和复发的理想指标。然而,并非所有PLC患者都会大量分泌AFP和GGT,这影响了仅通过监测这两种肿瘤标志物来评估PLC的准确性。分化簇3和161双阳性自然杀伤T(CD3CD161NKT)细胞亚群是一类与免疫功能以及肿瘤发生发展密切相关的分子。本研究旨在探讨CD3CD161NKT细胞亚群联合肿瘤标志物AFP和GGT在PLC患者诊断中的临床意义。

目的

探讨PLC患者外周血中CD3CD161NKT细胞亚群以及AFP和GGT变化的临床意义。

方法

PLC组包括2022年7月至2023年12月期间我院收治的30例确诊为PLC的患者,而对照组由我院30例接受常规体检的健康个体组成。采集两组患者的外周血样本。采用流式细胞术检测CD4NKT、CD8NKT、CD3CD56NKT、CD8CD56NKT、CD3CD161NKT和CD3CD161NKT的水平。使用全自动免疫分析仪测定血清AFP含量,并用全自动生化分析仪测定血清GGT含量。通过受试者工作特征曲线分析评估CD3CD161NKT细胞亚群以及AFP和GGT水平变化对PLC的诊断价值。

结果

两组患者的白细胞、中性粒细胞和血小板计数以及血尿素氮和血清肌酐水平均无显著差异(>0.05)。PLC组的淋巴细胞、红细胞、血红蛋白、总蛋白、白蛋白和球蛋白水平低于对照组,而谷丙转氨酶、谷草转氨酶和癌胚抗原水平高于对照组,差异具有统计学意义(<0.05)。两组外周血CD4NKT、CD8NKT和CD3CD56NKT细胞无显著差异(>0.05)。PLC组中CD8CD56NKT细胞(8.35%±1.01%)、CD3CD161NKT细胞(14.36%±1.55%)和CD3CD161NKT细胞(12.08%±1.34%)的百分比高于对照组(<0.05)。PLC组的AFP(335.71±20.89 ng/mL)和GGT(136.87±15.62 U/mL)水平高于对照组(<0.05)。CD8CD56NKT、CD3CD161NKT、CD3CD161NKT、AFP和GGT单独诊断PLC的敏感性分别为70.00%、83.33%、80.00%、56.67%和53.33%(<0.05),特异性分别为66.67%、80.00%、76.67%、76.67%和66.67%(<0.05)。联合检测的曲线下面积为0.898,敏感性为86.67%,特异性为80.00%(<0.05)。

结论

PLC患者外周血中CD8CD56NKT、CD3CD161NKT、CD3CD161NKT、AFP和GGT水平显著升高。这五项指标联合检测可提高PLC诊断的敏感性和特异性,为PLC的早期临床诊断提供有力依据。

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