UMR 1019 Human Nutrition Unit, INRAe, University of Clermont Auvergne, CRNH Auvergne, 63000, Clermont-Ferrand, France.
Faculty of Sciences II, Lebanese University, Fanar, Lebanon.
J Physiol Biochem. 2022 May;78(2):335-342. doi: 10.1007/s13105-021-00868-z. Epub 2022 Jan 5.
Human cathelicidin refers to the cationic antimicrobial peptide hCAP18/LL-37. LL-37 is formed by cleavage of the propeptide hCAP18 coded by the CAMP gene. The active form of vitamin D, 1,25-dihydroxyvitamin D (1,25(OH)D), has been shown to induce the CAMP gene expression through promoter activation. We previously failed to demonstrate in a clinical trial that supplementation of 25-hydroxyvitamin D (25(OH)D) improves LL-37 serum levels. The aim of this work was to evaluate the impact of 25(OH)D supplementation on intracellular expression of CAMP and secretion of LL-37 in an ex vivo model using the peripheral blood mononuclear cells (PBMC). PBMC collected from healthy donors and incubated with different concentrations of 25(OH)D (0 ng/ml: control (D0); 25 ng/ml: deficient (D25); 75 ng/ml: physiological (D75); 125 ng/ml: supraphysiological (D125)) were stimulated or not with lipopolysaccharide (LPS, 100 ng/ml) or synthetic double-stranded RNA Poly (I: C) (PIC, 10 µg/ml). The intracellular expressions of the CAMP gene and the hCAP18 peptide were measured respectively after 24-h and 48-h incubation periods. The concentration of LL-37 was determined in the culture medium after 48-h incubation. 25(OH)D significantly induced CAMP gene expression at 24 h with a maximum effect at a dose of D125 in either unstimulated (tenfold expression) or stimulated (LPS: 100-fold expression; PIC: 15-fold expression) conditions. Intracellular hCAP18 peptide was overexpressed at 48 h under unstimulated (1.5-fold, D125) and stimulated conditions, LPS (twofold, D125) and PIC (2.5-fold, D125). The secretion of LL-37 in the culture medium was significantly induced by 25(OH)D only in both stimulated (LPS and PIC) conditions in a dose-dependent manner. Our results demonstrate that 25(OH)D incubation increases intracellular expression of CAMP and hCAP18, but extracellular secretion of LL-37 antimicrobial peptide is increased by 25(OH)D only when PBMC from healthy donors were stimulated with bacterial or viral immune mimetic.
人源防御素是指阳离子抗菌肽 hCAP18/LL-37。LL-37 是由 CAMP 基因编码的前肽 hCAP18 裂解而成的。活性形式的维生素 D,1,25-二羟维生素 D(1,25(OH)D)已被证明可通过启动子激活诱导 CAMP 基因表达。我们之前在一项临床试验中未能证明补充 25-羟维生素 D(25(OH)D)可改善 LL-37 血清水平。本研究的目的是使用外周血单核细胞(PBMC)在体外模型中评估 25(OH)D 补充对 CAMP 细胞内表达和 LL-37 分泌的影响。从健康供体采集 PBMC,分别用不同浓度的 25(OH)D(0ng/ml:对照(D0);25ng/ml:缺乏(D25);75ng/ml:生理(D75);125ng/ml:超生理(D125))孵育,然后用脂多糖(LPS,100ng/ml)或合成双链 RNA Poly(I:C)(PIC,10μg/ml)刺激或不刺激。分别在孵育 24 小时和 48 小时后测量 CAMP 基因和 hCAP18 肽的细胞内表达。在孵育 48 小时后测定培养基中 LL-37 的浓度。25(OH)D 在未刺激(D125 时为 10 倍表达)或刺激条件下(LPS:100 倍表达;PIC:15 倍表达)均显著诱导 CAMP 基因在 24 小时时表达,最大作用剂量为 D125。在未刺激(D125 时为 1.5 倍)和刺激条件下(LPS:D125 时为两倍;PIC:D125 时为 2.5 倍),hCAP18 肽在细胞内过度表达 48 小时。只有在 PBMC 受到细菌或病毒免疫模拟物刺激时,25(OH)D 才能以剂量依赖性方式显著诱导培养基中 LL-37 抗菌肽的分泌。
我们的研究结果表明,25(OH)D 孵育可增加 CAMP 和 hCAP18 的细胞内表达,但仅当来自健康供体的 PBMC 受到细菌或病毒免疫模拟物刺激时,25(OH)D 才会增加 LL-37 抗菌肽的细胞外分泌。
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