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在哺乳期大鼠中通过脂质氨基糖苷衍生物进行miRNA的口服递送。

Oral Delivery of miRNA With Lipidic Aminoglycoside Derivatives in the Breastfed Rat.

作者信息

Beuzelin Diane, Pitard Bruno, Kaeffer Bertrand

机构信息

UMR 1280, NUN, Institut National de la Recherche Agronomique, Nantes, France.

Centre de Recherche en Cancérologie et Immunologie Nantes Angers (CRCINA), Institut National de la Santé et de la Recherche Médicale (INSERM), Université d'Angers, Université de Nantes, Nantes, France.

出版信息

Front Physiol. 2019 Aug 13;10:1037. doi: 10.3389/fphys.2019.01037. eCollection 2019.

Abstract

CONTEXT

Specific targeting of endogenous miRNAs which are involved in epigenetics, may help understanding homeostasis with therapeutic benefits. We use new biologically inspired vehicles consisting of lipoaminoglycosides to deliver mir-320-3p, a known human breast milk exosomal miRNA, or its antagomiR.

MATERIALS AND METHODS

Four lipoaminoglycosides were screened for cytotoxicity and their biophysical properties. 1-h breast-restricted rats received single-oral treatment of either the lipoaminoglycoside Dioleyl-Succinyl Paromomycin (DOSP) complexed with miRNA or antagomiR, or of control medium at the light on (ZeitGeber Time: ZT-0H) or off (ZT-12H). Glycemia, triglycerides, cholesterol, free-fatty acid were assayed at 0, 4, 8, and 12 h post-treatment. In the stomach, small intestine, liver, plasma, adipose tissue, plexus choroid, and cortex, relevant miRNA with precursors and mRNA (polr3d, hspb6, c-myc, stat1, clock, bmal1, per1, npas2, sirt1-6, and cyclinD1) were quantified by q-PCR. Expression of POLR3D and HSPB6 proteins were analyzed in stomach and liver by Western blot. Immunoprecipitations with anti-AGO1 and 2 were performed on nuclear and cytoplasmic fractions of gastric cells along with detection of miRNA-320-3p in nucleoli. Chromatin ImmunoPrecipitation with anti-Trimethyl-histone-3-Lys-4 and Lys-27 detecting the polr3d promoter and miR-320-3p, were performed for all groups.

RESULTS

Selected DOSP (diameter: 80-200 nm) did not alter gastric extracellular vesicle secretion a few hours after intake. The miR-320-3p was mainly found in gastric or small intestinal cells, reaching the blood and liver in low amount. We have found significant up-regulation of polr3d mRNA (ANOVA, < 0.0001) at ZT-20H for the miR-320-3p-supplemented group and a higher expression of POLR3D for antagomiR group (ANOVA, < 0.05). We had a low accumulation of miR-320-3p at ZT-20H in nucleoli, without stat1 evolution. Delivering a high amount of miRNA or antagomiR disrupts RNA-Induced Silencing Complexes in cytoplasm triggering some transfer of extracellular molecules into nuclei with alteration of immune complexes on the polr3d promoter (with a higher amount found in the K4 histone-3-me3 immune complexes at ZT-20H).

CONCLUSION

Extracellular miRNAs embedded in DOSP have a rapid impact on RNAi and on nuclear chromatin complexes depending on the daily rhythm. An integrative view of the impact of extracellular miRNA on physiology will improve assaying epigenetic manipulations following nutritional stress.

摘要

背景

特异性靶向参与表观遗传学的内源性微小RNA(miRNA),可能有助于理解内环境稳态并带来治疗益处。我们使用由脂氨基糖苷组成的新型生物启发式载体来递送mir - 320 - 3p(一种已知的人母乳外泌体miRNA)或其拮抗剂。

材料与方法

筛选了四种脂氨基糖苷的细胞毒性及其生物物理性质。对1小时禁食的大鼠在光照时(时间geber时间:ZT - 0H)或光照结束时(ZT - 12H)进行单次口服治疗,分别给予与miRNA或拮抗剂复合的脂氨基糖苷二油酰琥珀酰巴龙霉素(DOSP),或对照培养基。在治疗后0、4、8和12小时测定血糖、甘油三酯、胆固醇、游离脂肪酸。通过q - PCR对胃、小肠、肝脏、血浆、脂肪组织、脉络丛和皮质中的相关miRNA及其前体和mRNA(polr3d、hspb6、c - myc、stat1、clock、bmal1、per1、npas2、sirt1 - 6和细胞周期蛋白D1)进行定量。通过蛋白质印迹法分析胃和肝脏中POLR3D和HSPB6蛋白的表达。对胃细胞的核和细胞质部分进行抗AGO1和2的免疫沉淀,并同时检测核仁中的miRNA - 320 - 3p。对所有组进行用抗三甲基组蛋白 - 3 - 赖氨酸 - 4和赖氨酸 - 27检测polr3d启动子和miR - 320 - 3p的染色质免疫沉淀。

结果

摄入后数小时,选定的DOSP(直径:80 - 200 nm)未改变胃细胞外囊泡的分泌。miR - 320 - 3p主要存在于胃或小肠细胞中,少量到达血液和肝脏。我们发现,对于补充miR - 320 - 3p的组,在ZT - 20H时polr3d mRNA有显著上调(方差分析,< 0.0001),而对于拮抗剂组,POLR3D表达更高(方差分析,< 0.05)。在ZT - 20H时,miR - 320 - 3p在核仁中的积累较低,stat1无变化。递送大量的miRNA或拮抗剂会破坏细胞质中的RNA诱导沉默复合体,触发一些细胞外分子转移到细胞核中,同时改变polr3d启动子上的免疫复合体(在ZT - 20H时,在K4组蛋白 - 3 - me3免疫复合体中发现的量更高)。

结论

嵌入DOSP的细胞外miRNA根据每日节律对RNA干扰和核染色质复合体有快速影响。细胞外miRNA对生理学影响的综合观点将改善对营养应激后表观遗传操作的检测。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/00ca/6700720/645dc1e1bdf6/fphys-10-01037-g001.jpg

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