刚地弓形虫棒状体蛋白16过表达人单核THP-1细胞的转录组学分析

doi:10.12140/j.issn.1000-7423.2025.03.002

中国寄生虫学与寄生虫病杂志 ›› 2025, Vol. 43 ›› Issue (3): 317-323.doi: 10.12140/j.issn.1000-7423.2025.03.002

刚地弓形虫棒状体蛋白16过表达人单核THP-1细胞的转录组学分析

李佳铭¹^,²^,³()(), 陈梅⁴, 党甜甜¹^,²^,³, 殷荷¹^,²^,³, 赵志军¹^,²^,³^,^*()()

1 宁夏医科大学总医院医学实验中心，宁夏银川 750004
2 宁夏临床病原微生物重点实验室，宁夏银川 750004
3 宁夏医学检验临床研究中心，宁夏银川 750004
4 仁怀市人民医院检验科，贵州遵义 564507

收稿日期:2024-11-15 修回日期:2025-01-07 出版日期:2025-06-30 发布日期:2025-06-25
通讯作者: *赵志军（ORCID：0000-0001-7645-996），男，博士，研究员，从事临床病原微生物与免疫学研究。E-mail：z15815z@163.com
作者简介:李佳铭（ORCID：0009-0003-6795-3658），女，硕士，技师，从事临床病原微生物与免疫学研究。E-mail：1151143915@qq.com
基金资助:
中央引导地方科技发展专项(2024FRD05043);宁夏回族自治区重点研发计划(2023BEG02002)

Transcriptome analysis of human monocytic THP-1 cells overexpressing Toxoplasma gondii rhoptry protein 16

LI Jiaming¹^,²^,³()(), CHEN Mei⁴, DANG Tiantian¹^,²^,³, YIN He¹^,²^,³, ZHAO Zhijun¹^,²^,³^,^*()()

1 Medical Laboratory Center, General Hospital of Ningxia Medical University, Yinchuan 750004, Ningxia,China
2 Key Laboratory of Clinical Pathogenic Microorganisms of Ningxia, Yinchuan 750004, Ningxia,China
3 Clinical Research Center of Medical Laboratory of Ningxia, Yinchuan 750004, Ningxia, China
4 Department of Laboratory, Renhuai People’s Hospital, Zunyi 564507, Guizhou, China

Received:2024-11-15 Revised:2025-01-07 Online:2025-06-30 Published:2025-06-25
Contact: *E-mail: z15815z@163.com
Supported by:
Central Guided Local Science and Technology Development Special Project(2024FRD05043);Key Research and Development Program of Ningxia Hui Autonomous Region(2023BEG02002)

摘要/Abstract

摘要：

目的转录组测序分析Ⅰ型RH株刚地弓形虫棒状体蛋白16（ROP16）过表达人单核THP-1细胞的基因表达谱变化，筛选免疫应答相关驱动基因。方法将人单核THP-1细胞接种于96孔板，过表达组中加入ROP16过表达慢病毒，对照组加入等量培养基，72 h后在荧光显微镜下观察转染情况。TRIzol法提取过表达组和对照组人单核THP-1细胞总RNA，并进行转录组测序，筛选差异表达基因（DEG），绘制火山图。对DEG进行聚类分析、京都基因与基因组百科全书（KEGG）代谢通路富集分析和基因本体（GO）功能富集分类，筛选出过表达组和对照组的DEG，并进行实时荧光定量PCR（qPCR）验证。两组间比较采用独立样本t检验。结果荧光显微镜下过表达组90%以上的人单核THP-1细胞表达绿色荧光，对照组细胞未见绿色荧光。qPCR结果表明，过表达组ROP16 mRNA相对转录水平（1 083.484 ± 68.990）较对照组（1.000 ± 0）显著上调（t = 22.9，P < 0.01），表明已构建稳定表达ROP16的THP-1细胞株。共筛选出312个DEG，其中193个表达上调，119个表达下调。KEGG注释结果显示，注释到有机体系统的DEG占比最高（24.2%），显著富集于85个条目，其中免疫系统显著富集的基因有47个。KEGG富集分析发现，DEG富集至20条信号通路上，Th1和Th2细胞分化、自然杀伤细胞介导的细胞毒性及IL-17信号通路等3条与免疫系统相关的通路分别富集DEG 6、7和8个。GO功能注释结果显示，共有309个DEG注释到生物过程、细胞组分和分子功能等3个一级节点分类下的55个二级节点分类中。GO富集结果显示，DEG显著富集于炎症反应、肿瘤坏死因子产物负调控、细胞因子产生、γ干扰素产生的正调节，以及与免疫应答相关的通路中。qPCR检测发现ROP16过表达组中MAN2B1、FOS、C1QA的mRNA相对转录水平（25.994 ± 0.382、60.584 ± 2.968、 36.759 ± 0.180）均高于对照组（1.000 ± 0.039、1.000 ± 0.015、1.000 ± 0）（t = 92.00、28.39、280.7，P < 0.05或0.01），LMNB1、IL-6和 IL-12 mRNA相对转录水平（0.728 ± 0.054、0.517 ± 0.073、0.587 ± 0.015）均低于对照组（1.052 ± 0.027、1.000 ± 0.039、1.000 ± 0.010）（t = 7.64、8.24、33.62，P < 0.05或0.01）。结论 Ⅰ型RH株弓形虫效应分子ROP16过表达后，人单核THP-1细胞基因表达谱发生了明显变化。

关键词: 刚地弓形虫, 棒状体蛋白16, 人单核THP-1细胞, 转录组, 免疫应答

Abstract:

Objective To investigate the changes in the gene expression profile of human monocyte THP-1 cells overexpressing Toxoplasma gondii rhoptry protein 16 (ROP16) using transcriptome sequencing, and to screen immune response-related driver genes. Methods Human monocytic THP-1 cells were seeded onto 96-well plates. Cells in the overexpression group was transfected with ROP16 overexpression lentivirus for 72 h, and cells in the control group were treated with an equal volume of culture medium. The efficiency of cell transfection was checked under a fluorescence microscope. Total RNA was extracted from THP-1 cells and THP-1 cells stably expressing ROP16 using the TRIzol reagent, followed by transcriptome sequencing. Differentially expressed genes (DEG) were screened, and a volcano plot was generated. DEGs were subjected to cluster analysis, Kyoto encyclopedia of genes and genomes (KEGG) metabolic pathway enrichment analysis, and gene ontology (GO) functional enrichment classification to screen immune response-related driver genes in human monocytic THP-1 cells following T. gondii infections, and gene expression was quantified using qPCR assay. Differences of means between groups were tested for statistical significance with independent sample t-test. Results Fluorescence microscopy displayed green fluorescence in more than 90% of the cells in the overexpression group in each field of view, and no green fluorescence was observed in the control group. qPCR assay quantified a higher relative expression level of ROP16 mRNA in the overexpression group (1 083.484 ± 68.990) than in the control group (1.000 ± 0) (t = 22.9, P < 0.01), indicating the successful generation of THP-1 cells that stably expressed ROP16. A total of 312 DEGs were identified in THP-1 cells stably expressing ROP16, including 193 upregulated genes and 119 downregulated genes. KEGG annotations showed that the highest proportion of DEGs were annotated to the organism system (24.2%), with 85 items significantly enriched, among which 47 genes were significantly enriched in the immune system. KEGG enrichment analysis showed that DEGs were significantly enriched in 20 signaling pathways, and 6, 7, and 8 DEG were significantly enriched in three pathways related to the immune system, including Th1 and Th2 cell differentiation, natural killer cell-mediated cytotoxicity, and IL-17 signaling pathways, respectively. GO functional annotations showed that a total of 309 DEGs were annotated to 55 secondary node classifications under three primary node classifications of biological processes, cellular components, and molecular functions. GO enrichment analysis showed that DEGs were significantly enriched in inflammatory response, negative regulation of tumor necrosis factor products, cytokine production, positive regulation of interferon-γ production, and immune response-related pathways. RT-qPCR assay detected that higher relative expression of MAN2B1, FOS, C1QA mRNA (25.994 ± 0.382、60.584 ± 2.968、 36.759 ± 0.180) in cells in the ROP16 overexpression group than in the control group (1.000 ± 0.039、1.000 ± 0.015、1.000 ± 0) (t = 92.00, 28.39, 280.7, P < 0.05 or 0.01), and lower relative expression of LMNB1, IL-6, and IL-12 mRNA (0.728 ± 0.054, 0.517 ± 0.073, 0.587 ± 0.015) in the overexpression group than in the control group (1.052 ± 0.027、1.000 ± 0.039、1.000 ± 0.010) (t = 7.64, 8.24, 33.62, P < 0.05 or 0.01). Conclusion The gene expression profile of human monocyte THP-1 cells changes significantly and may play important roles in the immune response following T. gondii infection.

Key words: Toxoplasma gondii, Rhoptry protein 16, Human monocytic THP-1 cell, Transcriptome, Immune response

中图分类号:

R382.5

李佳铭, 陈梅, 党甜甜, 殷荷, 赵志军. 刚地弓形虫棒状体蛋白16过表达人单核THP-1细胞的转录组学分析[J]. 中国寄生虫学与寄生虫病杂志, 2025, 43(3): 317-323.

LI Jiaming, CHEN Mei, DANG Tiantian, YIN He, ZHAO Zhijun. Transcriptome analysis of human monocytic THP-1 cells overexpressing Toxoplasma gondii rhoptry protein 16[J]. Chinese Journal of Parasitology and Parasitic Diseases, 2025, 43(3): 317-323.

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基因名称 Gene name	引物序列（5'→3'） Primer sequence（5'→3'）
甘油醛-3-磷酸脱氢酶GAPDH	F：CAGGAGGCATTGCTGATGAT
甘油醛-3-磷酸脱氢酶GAPDH	R：GAAGGCTGGGGCTCATTT
棒状体蛋白 ROP-16	F：TGGGCTCCTGAACTTGCGAAATC
棒状体蛋白 ROP-16	R：AGACGAACTCGAAGATTGCCAACC
组织蛋白酶B CTSB	F：GGTGGCCTCTAYGAATCCCA
组织蛋白酶B CTSB	R：GCCAGGTCACAGATCTTGCTA
原癌基因 Fos FOS	F：GACTGATACACTCCAAGCGG
原癌基因 Fos FOS	R：CAGGGATCTTGCAGGCAGGT
核纤层蛋白B1 LMNB1	F：CTGAGGCGGAATGAGAGATGC
核纤层蛋白B1 LMNB1	R：CTGAGGCGGAATGAGAGATGC
甘露糖苷酶α 2B成员1 MAN2B1	E：GGAGGCGGAATGAGAGATGC
甘露糖苷酶α 2B成员1 MAN2B1	R：CTGTCTGTGTAGAAGCGTCCC
补体C1q B链 C1QB	F：ACAGTAGGGCTTGGTGAATG
补体C1q B链 C1QB	R：GCTGGGACACAGAGTTGAAT
组织蛋白酶A CTSA	F：CATCTTCACTCGCCTGCCAC
组织蛋白酶A CTSA	R：CGGGTTGTTGAGGTAGGTGG
S100钙结合蛋白A8 S100A8	F：CTCTATCATCGACGTCTACC
S100钙结合蛋白A8 S100A8	R：ATCATGGAGGACCTGGACAC
S100A9	F：ATCATGGAGGACCTGGACAC
S100A9	R：ACCCTCGTGCATCTTCTCGT
C1QA	F：CCGGCTACTACTACTTCACC
C1QA	R：CCTTGTTGGTGGTGTCACAG
C1QC	F：TGCACCCAACAGCCTGATCA
C1QC	R：GCGACGCGTGGTAGACAAAG
白细胞介素1β IL-1β	F：ATGGCTTATTACAGTGGCAATGAG
白细胞介素1β IL-1β	R：GTAGTGGTGG TCGGAGATTCG
IL-18	F：GCTGAAGATGATGAAAACCTGG
IL-18	R：CAAATAGAGGCCGATTTCCTTG
IL-10	F：GCCAAGCCTTGTCTGAGATGATCC
IL-10	R：AATCGATGACAGCGCCGTAGC
IL-12	F：GAGGTCCCTCCAAACCGTTGTC
IL-12	R：GATGTAATAGTCCCATCCTTCTTT
IL-6	F：GCCAGAGCTGTGCAGATGAGTAC
IL-6	R：AGTGGCATTGCATCCCTGAGTTG
IL-17	F：TCCCCATCCAGCAAGAGATCCTG
IL-17	R：AGCCCACGGACACCAGTATCTTC
肿瘤坏死因子α TNF-α	F：TCTCCTTCCTGATCGTGGCA
肿瘤坏死因子α TNF-α	R：GGCTACAGGCTTGTCACTCG
转化生长因子β TGF-β	F：AGCAACAATTCCTGGCGATACCTC
转化生长因子β TGF-β	R：TCAACCACTGCCGCACAACTC

基因 Gene	ROP16过表达组 ROP16 overexpression group	对照组 Control group
组织蛋白酶B CTSB	32.226 ± 0.632	1.000 ± 0.015
原癌基因Fos FOS	60.584 ± 2.968	1.000 ± 0.015
核纤层蛋白B1 LMNB1	0.728 ± 0.054	1.052 ± 0.027
甘露糖苷酶α 2B成员 MAN2B1	25.994 ± 0.382	1.000 ± 0.039
补体C1q B链 C1QB	52.166 ± 0.511	1.000 ± 0
C1QA	36.759 ± 0.180	1.000 ± 0
CTSA	3.580 ± 0.035	1.001 ± 0.044
S100钙结合蛋白A8 S100A8	13.693 ± 0.403	1.003 ± 0.108
S100A9	41.434 ± 3.651	1.001 ± 0.064
C1QC	23.837 ± 0.467	1.001 ± 0.059
白细胞介素1β IL-1β	2.462 ± 0.277	1.000 ± 0.010
IL-18	1.454 ± 0.036	1.002 ± 0.093
IL-10	1.718 ± 0.076	1.000 ± 0
IL-12	0.587 ± 0.014	1.000 ± 0.010
IL-6	0.517 ± 0.073	1.000 ± 0.039
IL-17	1.366 ± 0.007	1.000 ± 0.025
肿瘤坏死因子α TNF-α	1.235 ± 0.012	1.000 ± 0.014
转化生长因子β TGF-β	14.124 ± 0.138	1.016 ± 0.251

刚地弓形虫棒状体蛋白16过表达人单核THP-1细胞的转录组学分析

Transcriptome analysis of human monocytic THP-1 cells overexpressing Toxoplasma gondii rhoptry protein 16

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