热物理场中复合抗菌肽对枯草芽孢杆菌芽孢的杀灭作用

朱改丽; 刘燚畅; 田鹏; 张浩杰; 章中

doi:10.13386/j.issn1002-0306.2025040376

热物理场中复合抗菌肽对枯草芽孢杆菌芽孢的杀灭作用

Inactivation of Bacillus subtilis Spores by Compound Antimicrobial Peptides in Thermal Physical Field

摘要

摘要: 细菌芽孢是食品中常见微生物，因其具有极端抗性而难以彻底被杀灭。本文旨在探究热物理场中（80、90 ℃）尼生素（Nisin）和ε-聚赖氨酸（ε-polylysine，ε-PL）复配使用对枯草芽孢杆菌芽孢的协同杀灭效果及其机制，为食品防腐保鲜提供更有效的方法。以OD_{600 nm}、OD_{260 nm}、OD_{280 nm}的变化表征芽孢内容物的释放及内膜损伤情况。利用扫描电镜观察芽孢形态结构的变化，采用傅里叶变换红外光谱法分析芽孢内膜脂质相态、蛋白质二级结构及核酸骨架的变化，测定Na⁺/K⁺-ATP酶活力以评估代谢状态。结果表明：90 ℃热处理下，添加0.5 g/L Nisin、0.25 g/L ε-PL处理后，分别可杀灭1.59 lg CFU/mL和1.22 lg CFU/mL的芽孢，而0.5 g/L Nisin复配0.25 g/L ε-PL使用后可杀灭4.28 lg CFU/mL的芽孢。经上述复配处理后，扫描电镜显示芽孢聚集现象显著加剧。2,6-吡啶二羧酸（2,6-dipicolinic acid, DPA）泄漏率高达76.03%，表明内膜严重受损。傅里叶变换红外光谱表明：芽孢内膜脂质相态由凝胶态转变为液晶态，核酸骨架被破坏，蛋白质二级结构含量发生显著改变（P<0.05），α螺旋和β折叠含量减少，而β转角及无规卷曲含量分别增加至43.81%和35.37%。此外，Na⁺/K⁺-ATP酶活力显著下降至最低值6.53 μmol/h/mg（P<0.05），芽孢能量代谢受到严重抑制。Nisin和ε-PL协同杀灭芽孢的机制主要在于：Nisin破坏芽孢内膜结构，内膜受损会导致芽孢核心水化，DPA等关键物质泄漏，ε-PL则通过受损的内膜进入芽孢核心，破坏DNA结构，最终导致芽孢死亡。

Abstract: Bacterial spores are common microbes in foods. They are difficult to be inactivated because of their extreme resistances. The synergistic inactivation effects and mechanism of Nisin combined with ε-polylysine treatment on Bacillus subtilis spores in thermal physical field (80, 90 ℃) were studied, and a more effective method for food preservation was provided. The changes of OD_{600 nm}, OD_{260 nm}, OD_{280 nm} values were used for characterizing the inner membrane damage and intracellular components release. Scanning electron microscope (SEM) was used for observing the changes in spore morphology and structure. Fourier transform infrared (FTIR) spectroscopy was used for analyzing the changes in lipids phase of spore inner membrane, the secondary structure of spore proteins, and nucleic acid backbone. The activity of Na⁺/K⁺-ATPase was determined to evaluate spore’s metabolic condition. The results are as follows: under 90 ℃ treatment, 1.59 lg CFU/mL or 1.22 lg CFU/mL Bacillus subtilis spores were inactivated respectively with addition of 0.5 g/L Nisin or 0.25 g/L ε-polylysine, while 4.28 lg CFU/mL spores were inactivated with combined usage of 0.5 g/L Nisin and 0.25 g/L ε-polylysine. After the combined treatment, SEM images indicated that the aggregation of spores significantly intensified. The 2,6-dipicolinic acid (DPA) release raised up to 76.03%, indicating serious inner membrane damage. FTIR spectroscopy indicated that the lipids in the spore inner membrane changed from a gel state to a liquid crystal state, nucleic acid backbone was damaged, and the content of secondary structures in proteins changed (P<0.05), the α-helix and β-folding content decreased, while the β-turn and random coil content increased respectively to 43.81% and 35.37%. In addition, the activity of Na⁺/K⁺-ATPase significantly decreased to lowest value 6.53μmol/h/mg (P<0.05), and the energy metabolism of spores was severely inhibited. The main mechanism of synergistic spore inactivation by Nisin and ε-polylysine was as follows: Nisin destroyed the inner membrane structure of spores, which resulted in core hydration and release of key components such as DPA. ε-polylysine penetrated the damaged inner membrane, entered the spore core, destroyed DNA structure, and finally caused spore inactivation.

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