Effect of ultraviolet radiation on expression of transient receptor potential ankyrin 1 in HaCaT cells

Liu Ying; Zhang Ting; Zhao Guangming; Ni Jing; Wang Yupeng; Liu Yuejian; Song Zhiqi

doi:10.3760/cma.j.issn.0412-4030.2017.10.004

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紫外线对HaCaT细胞中瞬时受体电位锚蛋白1的影响

中华皮肤科杂志, 2017,50(10) : 710-714. DOI: 10.3760/cma.j.issn.0412-4030.2017.10.004

摘要

目的

探讨HaCaT细胞中瞬时受体电位锚蛋白1（TRPA1）的光控作用及其机制。

方法

培养的HaCaT细胞分为225 mJ/cm² UVA刺激组和25 mJ/cm² UVB刺激组，UVA刺激组分为空白对照组（仅有HaCaT细胞）、视黄醛组、UVA组、视黄醛+ UVA组（UVA-TRPA1对照组）、视黄醛+ UVA+肉桂醛组（UVA-TRPA1激动组）、视黄醛+ UVA+樟脑组（UVA-TRPA1抑制组）；UVB刺激组分为空白对照组（仅有HaCaT细胞）、视黄醛组、UVB组、视黄醛+ UVB组（UVB-TRPA1对照组）、视黄醛+ UVB+肉桂醛组（UVB-TRPA1激动组）、视黄醛+ UVB+樟脑组（UVB-TRPA1抑制组）。qPCR、Western印迹检测HaCaT细胞中TRPA1的表达。流式细胞仪检测各组HaCaT细胞钙离子内流的变化。

结果

qPCR和Western印迹显示，HaCaT细胞中有TRPA1 mRNA及蛋白的表达。UVA作用后空白对照组、视黄醛组、UVA组、视黄醛+ UVA组荧光强度分别为155.06 ± 7.62、148. 37 ± 18.77、166.92 ± 3.71、331.333 ± 40.563，组间差异有统计学意义（F= 44.509，P < 0.01）。UVB作用后空白对照组、视黄醛组、UVB组、视黄醛+ UVB组荧光强度分别为150.20 ± 1.73、171.66 ± 56.23、147.56 ± 6.60、250.44 ± 9.13，组间差异有统计学意义（F= 85.261，P < 0.01），视黄醛+ UVA/UVB组荧光强度均高于空白对照组（q值分别为18.442、6.052，P < 0.01）。TRPA1激动剂和拮抗剂可调节UVA、UVB所引起的钙离子内流的变化（P<0.001），在UVA、UVB作用下，TRPA1激动剂组荧光强度均高于对照组（q值分别为14.934、32.770，P < 0.001），TRPA1抑制剂组荧光强度均低于对照组（q值分别为7.986、14.596，P < 0.001）。

结论

TRPA1在皮肤HaCaT细胞中有表达，UVA或UVB可通过TRPA1调控HaCaT细胞的钙离子内流。

引用本文: 刘影, 张婷, 赵光明, 等. 紫外线对HaCaT细胞中瞬时受体电位锚蛋白1的影响 [J] . 中华皮肤科杂志,2017,50 (10): 710-714. DOI: 10.3760/cma.j.issn.0412-4030.2017.10.004

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瞬时受体电位（transient receptor potential，TRP）通道是位于真核细胞膜上的一类重要的非选择性阳离子通道，最早发现于果蝇的视觉系统，突变体果蝇对持续的光刺激产生瞬时而非持续的峰电位^[1]。大多数TRP通道为钠离子、钙离子等渗透型通道，其中瞬时受体电位锚蛋白1（transient receptor potential ankyrin 1，TRPA1）为钙离子渗透型通道。Bellono等^[2,3]提出TRPA1可能是唯一的眼外光转导通路，表皮黑素细胞受到紫外线辐射时，Gα/q11蛋白-磷脂酶C信号转导途径被激活，随后激活TRPA1通道使大量的钙离子内流，从而导致早期黑素合成增加。为了进一步探讨TRPA1在角质形成细胞中的光控作用，我们研究了在长波紫外线（UVA）、中波紫外线（UVB）作用下，HaCaT细胞中视黄醛依赖性钙离子内流的情况以及TRPA1通道抑制及激活状态下对HaCaT细胞视黄醛依赖性钙离子内流的影响。

贡献者信息

刘影

116011　大连医科大学附属第一医院皮肤科

张婷

116011　大连医科大学附属第一医院皮肤科

赵光明

116011　大连医科大学附属第一医院皮肤科

倪静

116011　大连医科大学附属第一医院皮肤科

王宇鹏

116011　大连医科大学附属第一医院皮肤科

刘越坚

116011　大连医科大学附属第一医院中心实验室

宋智琦

116011　大连医科大学附属第一医院皮肤科

通信作者

宋智琦

116011　大连医科大学附属第一医院皮肤科

Email：szqdalian@163.com

关键词

角蛋白细胞; 紫外线; 瞬时受体电位通道; 锚蛋白类; HaCaT细胞;

基金项目

国家自然科学基金（81472865）

辽宁省自然科学基金（2014023005）

历史

出版日期：2017-10-15

收稿日期：2016-12-09

本文编辑

朱思维颜艳

Original Article

Effect of ultraviolet radiation on expression of transient receptor potential ankyrin 1 in HaCaT cells

Liu Ying, Zhang Ting, Zhao Guangming, Ni Jing, Wang Yupeng, Liu Yuejian, Song Zhiqi

Published 2017-10-15

Cite as Chin J Dermatol, 2017,50(10): 710-714. DOI: 10.3760/cma.j.issn.0412-4030.2017.10.004

Abstract

Objective

To investigate the photoregulation of transient receptor potential ankyrin 1 (TRPA1) in HaCaT cells, and to explore its mechanisms.

Methods

Cultured HaCaT cells were divided into 225-mJ/cm² UVA radiation groups and 25-mJ/cm² UVB radiation groups. HaCaT cells in the UVA radiation groups were further classified into 6 groups: blank control group 1 receiving no treatment, retinal group 1 treated with 12 μmol/L retinal alone, UVA group treated with 225 mJ/cm² UVA radiation alone, retinal+ UVA group (UVA-TRPA1 control group) , retinal+ UVA+ 500 μmol/L cinnamaldehyde group (UVA-TRPA1 agonist group) and retinal+ UVA+ 1 mmol/L camphor group (UVA-TRPA1 antagonist group) . Additionally, HaCaT cells in the UVB radiation groups were also further classified into 6 groups: blank control group 2 receiving no treatment, retinal group 2 treated with 12 μmol/L retinal alone, UVB group treated with 25-mJ/cm² UVB radiation, retinal+ UVB group (UVB-TRPA1 control group) , retinal+ UVB+ 500 μmol/L cinnamaldehyde group (UVB-TRPA1 agonist group) and retinal+ UVB+ 1 mmol/L camphor group (UVB-TRPA1 antagonist group) . Real-time fluorescence-based quantitative PCR (qPCR) and Western blot analysis were performed to determine the mRNA and protein expression of TRPA1 respectively. Flow cytometry was conducted to investigate changes of calcium influx in HaCaT cells in the above groups.

Results

qPCR and Western blot analysis showed that TRPA1 mRNA and protein were expressed in HaCaT cells. The fluorescence intensity of calcium influx significantly differed among the blank control group 1, retinal group 1, UVA group and retinal+ UVA group (155.06 ± 7.62, 148.37 ± 18.77, 166.92 ± 3.71 and 331.333 ± 40.563; F= 44.509, P < 0.01) , as well as among the blank control group 2, retinal group 2, UVB group and retinal+ UVB group (150.20 ± 1.73, 171.66 ± 56.23, 147.56 ± 6.60 and 250.44 ± 9.13; F= 85.261, P < 0.01) . Additionally, retinal+ UVA/UVB groups showed significantly higher fluorescence intensity of calcium influx compared with the blank control groups (q= 18.442, 6.052, P < 0.01) . The TRPA1 agonist cinnamaldehyde and its antagonist camphor could regulate the UVA-and UVB-induced calcium influx (P < 0.001) . Compared with the blank control group 1 and 2 respectively, the fluorescence intensity of retinal-dependent calcium influx was significantly higher in the UVA/UVB-TRPA1 agonist group (q= 14.934, 32.770, P < 0.001) , and significantly lower in the UVA/UVB-TRPA1 antagonist group (q= 7.986, 14.596, P < 0.001) .

Conclusion

TRPA1 is expressed in HaCaT cells, and UVA or UVB can regulate the calcium influx in HaCaT cells by adjusting the activity of TRPA1.

Key words:

Keratinocytes; Ultraviolet rays; Transient receptor potential channels; Ankyrins; HaCaT cells

Contributor Information

Liu Ying