中国儿童保健杂志 ›› 2014, Vol. 22 ›› Issue (4): 375-378.DOI: 10.11852/zgetbjzz2014-22-04-12

• 基础科研论著 • 上一篇    下一篇

n-3多不饱和脂肪酸对肥胖小鼠瘦素基因启动子区DNA甲基化的影响

王翠, 申文雯, 樊超男, 夏露露, 董华, 路媛媛, 齐可民   

  1. 首都医科大学附属北京儿童医院 北京市儿科研究所营养中心, 北京 100045
  • 收稿日期:2013-11-01 发布日期:2014-04-10 出版日期:2014-04-10
  • 通讯作者: 齐可民, E-mail:qkm732@sohu.com
  • 作者简介:王翠(1985-), 女, 河北人, 在读硕士, 研究方向为儿童营养。
  • 基金资助:
    荷兰Nutricia Research Foundation(2009-15, 2010-E4);北京市科委行业定额经费自主项目(2012-bjsekyjs-2)

Effect of n-3 polyunsaturated fatty on DNA methylation of the leptin promoter in obese mice.

WANG Cui, SHEN Wen-wen, FAN Chao-nan, XIA Lu-lu, DONG Hua, LU Yuan-yuan, QI Ke-min.   

  1. Clinical Nutrition Center, Beijing Pediatric Research Institute, Beijing Children's Hospital, Capital Medical University, Beijing 100045, China
  • Received:2013-11-01 Online:2014-04-10 Published:2014-04-10
  • Contact: QI Ke-min, E-mail:qkm732@sohu.com

摘要: 目的 从基因启动子区DNA甲基化环节, 探讨n-3多不饱和脂肪酸(n-3 polyunsaturated fatty acids, n-3 PUFAs)对肥胖状态下瘦素表达的表观遗传调控机制。方法 3~4周龄C57BL/6J雄性小鼠30只, 随机被分为3组(每组10只), 分别给予高脂饲料、鱼油n-3 PUFAs高脂饲料(脂肪含量均为34.9%, 供能比为40%)以及正常脂饲料(脂肪含量为4.3%, 供能比为10%)喂养4个月以诱导肥胖。喂养结束时取性腺周围脂肪组织, 应用RT-PCR检测脂肪组织瘦素mRNA水平;应用亚硫酸盐修饰直接测序(bisulfite sequencing-PCR, BSP)法检测瘦素基因启动子区CpG甲基化程度;应用染色质免疫共沉淀-荧光定量PCR(CHIP-RT-PCR)技术测定瘦素基因启动子区结合的DNA甲基化转移酶(DNMTs)、甲基化CpG结合蛋白2(MECP-2)以及RNA聚合酶2(Poly II)的变化。结果 与正常脂饲料组小鼠相比, 脂肪组织中瘦素mRNA 表达在高脂饲料诱导肥胖小鼠明显增加, 而在鱼油高脂饲料组肥胖小鼠无变化。基因启动子区甲基化结果显示, 高脂肥胖小鼠瘦素基因启动子区CpG位点甲基化程度、DNMT1、DNMT3a、DNMT3b和MECP-2含量均较正常饲料组显著升高, 并伴随Poly II含量减少;而鱼油高脂饲料组瘦素基因启动子区结合DNMT3a、DNMT3b and MeCP-2增加, 但启动子区MECP-2含量与高脂饲料组比缺有显著降低, DNMT1和Poly II以及CpG位点甲基化程度无改变。结论 肥胖状态下瘦素表达变化可能与基因启动子区DNA甲基化以及结合的相关调控蛋白、RNA聚合酶等有关;n-3 PUFAs对瘦素基因表达的调节也可能是通过对这些蛋白的影响而实现的。

关键词: n-3多不饱和脂肪酸, 肥胖, DNA甲基化, DNA甲基化转移酶, 甲基化CpG结合蛋白

Abstract: Obejective To investigate the epigenetic mechanisms linking n-3 polyunsaturated fatty acids (n-3 PUFAs) and the increased leptin expression in obesity. Methods Thirty 3~4 week-old male C57BL/6J mice were randomly divided into 3 groups and fed 4 months with two different high-fat diets (34.9% of fat providing 40% of total energy), high-fat diets (lard oil and sunflower oil) and fish oil high-fat diet (lard oil and fish oil), and one lean control diet (lard oil and sunflower oil, 4.3% of fat providing 10% of total energy).After fasted for 12 hours, mice were sacrificed and epididymal fat was collected.The mRNA expression of leptin in fat was assessed by real-time PCR (RT-PCR).Bisulfite sequencing-PCR (BSP) was used to determine the methylation level of CpG sites in the leptin promoter.Chromatin immunoprecipitation (ChIP) and RT-PCR were used to determine the amount of DNA methyltransferase (DNMTs), methyl CpG binding protein 2 (MeCP-2) and RNA polymerase II (Poly II) associated with the leptin promoter. Results As compared to the lean control diet group, the leptin mRNA expression in fat from the high-fat diet group was increased, whereas no change was found in the fish oil high-fat diet group.The methylation level of CpG sites in the leptin promoter and the associated proteins, DNMT1, DNMT3a, DNMT3b, MeCP-2 were higher than the lean control diet group with reduced binding of Poly II.In the fish oil high-fat group, increased DNMT3a, DNMT3b and MeCP-2 binding to the leptin promoter were found and the extent of MeCP-2 increase was less compared to the high-fat diet group.No changes were found in the associated DNMT1 and Poly II, and methylation of the leptin promoter in the fish oil high-fat diet group. Conclusion Our findings suggest that the leptin expression may be associated with the promoter methylation of the gene and the binding proteins and RNA polymerase in obesity, and n-3 PUFAs regulate the leptin expression through these pathways.

Key words: n-3 polyunsaturated fatty acids, obesity, DNA methylation, DNA methyltransferase, methyl CpG binding protein

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