产单核细胞李氏杆菌Lm4b_02325/26双基因缺失株构建及部分生物学特性试验

doi:10.11843/j.issn.0366-6964.2024.06.029

摘要/Abstract

摘要：

旨在构建食源性产单核细胞李氏杆菌毒力岛4(LIPI-4)中的抗转录终止子(Lm4b_02325)和未知蛋白(Lm4b_02326)基因的双缺失株，研究Lm4b_02325/26基因对产单核细胞李氏杆菌(Listeria monocytogenes，LM)的部分生物学特性的影响。利用同源重组技术构建LM928ΔLm4b_02325/26双缺失株，测定LM928和LM928ΔLm4b_02325/26双缺失株在脑心浸出液肉汤(brain heart infusion broth，BHI)、不同EtOH浓度、不同NaCl浓度、不同pH、不同温度下的D_{600 nm}，绘制生长曲线；RT-qPCR检测双基因缺失前后体外BHI培养环境下部分毒力因子转录水平；平板计数测定其对鼠巨噬细胞RAW264.7的黏附、侵袭与胞内增殖情况；感染C57BL/6小鼠后检测肝、脾、脑组织中的细菌数量。结果表明，成功构建具有遗传稳定性的双缺失株LM928ΔLm4b_02325/26。在含0.5%~10% NaCl或3%~4.5% EtOH的培养基中，双缺失株与野毒株生长没有明显差异，在pH=5条件下，双缺失株的生长率显著高于野毒株，pH=9条件下双缺失株的生长率显著低于野毒株。在不同温度(4 ℃、37 ℃、42 ℃)BHI培养基中，双缺失株与野毒株生长没有明显差异。Lm4b_02325/26基因双缺失株在BHI培养基中毒力因子hly、inlC和PlcA极显著上调(P < 0.01)，mpl、inlB、actA、inlP、PlcB、prfA、SigB、iap和inlA极显著下调(P < 0.01)；双缺失株对RAW264.7细胞的黏附率(14.86%)和侵袭率(2.23%)明显低于野毒株的黏附率(22.93%)和侵袭率(4.28%)(P < 0.01)；3、6、12 h时胞内增殖数量极显著低于野毒株(P < 0.01)；双缺失株与野毒株感染小鼠后，载菌量在肝、脾中没有显著差异，在脑组织中双缺失株载菌量为10⁴，高于野毒株的10^3.07，差异极显著(P < 0.01)。综上认为，LIPI-4的Lm4b_02325和Lm4b_02326基因参与LM毒力因子的表达和脑组织的定植能力，与弱酸强碱条件下适应力及对RAW264.7细胞的黏附、侵袭和胞内增殖有关。本研究为LIPI-4的功能研究奠定了基础。

关键词: 产单核细胞李氏杆菌, 双缺失株, 黏附侵袭, 胞内增殖, 载菌量, 生长曲线

Abstract:

The aim of this experiment was to construct a double-deletion strain of antitranscriptional terminator (Lm4b_02325) and unknown protein (Lm4b_02326) in Listeria pathogenicity island 4 (LIPI-4) of foodborne Listeria monocytogenes (LM). In order to study the effect of Lm4b_02325/26 gene on partial biological characteristics of LM. LM928ΔLm4b_02325/26 double-deletion strain was constructed by homologous recombination technology. The D_{600 nm} of LM928 and LM928ΔLm4b_02325/26 double-deletion strains were detected under BHI, different EtOH and NaCl concentrations, different pH and different temperatures, and the growth curves were plotted. The transcription level of some virulence factors of LM in BHI culture were detected by RT-qPCR. The adhesion, invasion and intracellular proliferation of LM-infected murine macrophages RAW264.7 were measured by plate count. And the bacterial load in liver, spleen and brain of C57BL/6 mice infected with LM intraperitoneal injection were detected. The results showed that, a genetically stable double-deletion strain LM928Δ Lm4b_02325/26 was successfully constructed. In the medium containing 0.5%~10% NaCl or 3%~4.5% EtOH, there was no significant difference between the growth of LM928ΔLm4b_02325/26 and LM928. The growth rate of LM928ΔLm4b_02325/26 strain was significantly higher than that of LM928 under the condition of pH5, and the growth rate of LM928Δ Lm4b_02325/26 strain was significantly lower than that of LM928 under the condition of pH9.In BHI medium at different temperatures (4 ℃, 37 ℃, 42 ℃), there was no significant difference between the growth of double-deficient strains and wild strains. The hly, inlC and PlcA genes of LM928Δ Lm4b_02325/26 strain in BHI were significantly upregulated (P < 0.01), while mpl, inlB, actA, inlP, PlcB, prfA, SigB, iap, and inlA genes were significantly downregulated (P < 0.01). The adhesion rate (14.86%) and invasion rate (2.23%) of LM928Δ Lm4b_02325/26 strain to RAW264.7 cells were significantly lower than those of wild strains (with adhesion rate of 22.93% and invasion rate of 4.28%) (P < 0.01). The number of bacteria in RAW264.7 cells infected by LM928Δ Lm4b_02325/26 strain was significantly lower than that of LM928 strain at 3, 6 and 12 h after infection (P < 0.01). In animal experiment, after the infection of mice, there was no significant difference in bacterial load between the two strains in the liver or spleen of mice, but in the brain tissue, the bacterial load of LM928Δ Lm4b_02325/26 strain was 10⁴, which was higher than that of the LM928 10^3.07, and the difference was extremely significant (P < 0.01). In summary, the Lm4b_02325 and Lm4b_02326 genes of LIPI-4 are involved in the expression of LM virulence factors and the colonization ability of brain tissues, and are related to adaptability under weak acid and strong base conditions and the adhesion, invasion and intracellular proliferation of LM to RAW264.7 cells. This study lays a base for the functional study of LIPI-4.

Key words: Listeria monocytogenes, double deletion strain, adhesion invasion, intracellular proliferation, bacterial load, growth curve

中图分类号:

S852.61

任慧杰, 马勋, 王静, 刘彩霞, 曾东东, 寇丽君, 史唯地, 吕双飞, 钱瑞宣, 高盛杰. 产单核细胞李氏杆菌Lm4b_02325/26双基因缺失株构建及部分生物学特性试验[J]. 畜牧兽医学报, 2024, 55(6): 2578-2587.

Huijie REN, Xun MA, Jing WANG, Caixia LIU, Dongdong ZENG, Lijun KOU, Weidi SHI, Shuangfei LÜ, Ruixuan QIAN, Shengjie GAO. Construction and Partial Biological Characteristics Trial of Lm4b_02325/26 Double Gene Deletion Strain of Listeria monocytogenes[J]. Acta Veterinaria et Zootechnica Sinica, 2024, 55(6): 2578-2587.

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引物 Primers	引物序列(5′→3′) Primer sequences(5′→3′)	酶切位点 Restriction site	扩增产物大小/bp Amplicon size	退火温度/℃ Annealing temperature
56-F1	AA$\underline{{\rm{CTGCAG}}}$GAACAGGTAATCGAAGCGAC	Pst I	488	58
56-R1	TCTCACTCCTTCAAACTGTCACTACTCCTTACT
56-F2	AGTAAGGAGTAGTGACAGTTTGAAGGAGTGAGA	EcoR I	339	58
56-R2	CG$\underline{{\rm{GAATTC}}}$CTAATCCATGCTTTAGTGGGA
56-DF	GTGGAGACCAAGAAGCTAGTT		3 997	58
56-DR	AGCCATAATTTTTAGCTAGTG		(1 318)

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