Zum Hauptinhalt springen
UB Hagen

Leptin relieves ischemia/reperfusion induced acute kidney injury through inhibiting apoptosis and autophagy.

Li, S ; Zhuang, K ; et al.
In: Zhong nan da xue xue bao. Yi xue ban = Journal of Central South University. Medical sciences, Jg. 47 (2022-01-28), Heft 1, S. 8-17
Online academicJournal
Zugriff:
Full Text Finder (Volltext)

Objectives: Acute kidney injury (AKI) can be caused by ischemia/reperfusion (I/R), nephrotoxin, and sepsis, with poor prognosis and high mortality. Leptin is a protein molecule that regulates the body's energy metabolism and reproductive activities via binding to its specific receptor. Leptin can inhibit cardiomyocyte apoptosis caused by I/R, but its effect on I/R kidney injury and the underlying mechanisms are still unclear. This study aims to investigate the effect and mechanisms of leptin on renal function, renal histopathology, apoptosis, and autophagy during acute I/R kidney injury.

Methods: Healthy adult male mice were randomly divided into 4 groups: a sham+wild-type mice (ob/+) group, a sham+leptin gene-deficient mice (ob/ob) group, an I/R+ob/+ group, and an I/R+ob/ob group ( n =8 per group). For sham operation, a longitudinal incision was made on the back of the mice to expose and separate the bilateral kidneys and renal arteries, and no subsequent treatment was performed. I/R treatment was ischemia for 30 min and reperfusion for 48 h. The levels of BUN and SCr were detected to evaluate renal function; HE staining was used to observe the pathological changes of renal tissue; TUNEL staining was used to observe cell apoptosis, and apoptosis-positive cells were counted; Western blotting was used to detect levels of apoptosis-related proteins (caspase 3, caspase 9), autophagy-related proteins [mammalian target of rapamycin (mTOR), phosphorylated mTOR (p-mTOR), LC3 I, LC3 II], mTOR-dependent signaling pathway proteins [phosphate and tension homology (PTEN), adenosine monophosphate-activated protein kinase (AMPK), protein kinase B (AKT), extracellular regulated protein kinase (ERK), phosphorylated PTEN (p-PTEN), phosphorylated AMPK (p-AMPK), phosphorylated AKT (p-AKT), phosphorylated ERK (p-ERK)].

Results: There was no significant difference in the levels of BUN and SCr between the sham+ob/+ group and the sham+ob/ob group (both P >0.05). The levels of BUN and SCr in the I/R+ob/+ group were significantly higher than those in the sham+ob/+ group (both P <0.05). Compared with the mice in the sham+ob/ob group or the I/R+ob/+ group, the levels of BUN and SCr in the I/R+ob/ob group were significantly increased (all P <0.05). There was no obvious damage to the renal tubules in the sham+ob/+ group and the sham+ob/ob group. Compared with sham+ob/+ group and sham+ob/ob group, both the I/R+ob/+ group and the I/R+ob/ob group had cell damage such as brush border shedding, vacuolar degeneration, and cast formation. Compared with the I/R+ob/+ group, the renal tubules of the mice in the I/R+ob/ob group were more severely damaged. The pathological score of renal tubular injury showed that the renal tubular injury was the most serious in the I/R+ob/ob group ( P <0.05). Compared with the sham+ob/+ group, the protein levels of caspase 3, caspase 9, PTEN, and LC3 II were significantly up-regulated, the ratio of LC3 II to LC3 I was significantly increased, and the protein levels of p-mTOR, p-PTEN, p-AMPK, p-AKT, and p-ERK were significantly down-regulated in the I/R+ob/+ group (all P <0.05). Compared with the sham+ob/ob group, the protein levels of caspase 3, caspase 9, PTEN, and LC3 II were significantly up-regulated, and the ratio of LC3 II to LC3 I was significantly increased, while the protein levels of p-mTOR, p-PTEN, p-AMPK, p-AKT, and p-ERK were significantly down-regulated in the I/R+ob/ob group (all P <0.05). Compared with the I/R+ob/+ group, the levels of p-mTOR, p-PTEN, p-AMPK, p-AKT were more significantly down-regulated, while the levels of caspase 3, caspase 9, PTEN, and LC3 II were more significantly up-regulated, and the ratio of LC3 II to LC3 I was more significantly increase in the I/R+ob/ob group (all P <0.05).

Conclusions: Renal function and tubular damage, and elevated levels of apoptosis and autophagy are observed in mice kidneys after acute I/R. Leptin might relieve I/R induced AKI by inhibiting apoptosis and autophagy that through a complex network of interactions between mTOR-dependent signaling pathways.

Titel:
Leptin relieves ischemia/reperfusion induced acute kidney injury through inhibiting apoptosis and autophagy.
Autor/in / Beteiligte Person: Li, S ; Zhuang, K ; He, Y ; Deng, Y ; Xi, J ; Chen, J
Link:
Zeitschrift: Zhong nan da xue xue bao. Yi xue ban = Journal of Central South University. Medical sciences, Jg. 47 (2022-01-28), Heft 1, S. 8-17
Veröffentlichung: Changsha Shi : "Zhong nan da xue xue bao (yi xue ban)" bian ji bu, 2004-, 2022
Medientyp: academicJournal
ISSN: 1672-7347 (print)
DOI: 10.11817/j.issn.1672-7347.2022.210244
Schlagwort:
  • AMP-Activated Protein Kinases metabolism
  • Animals
  • Apoptosis
  • Apoptosis Regulatory Proteins metabolism
  • Apoptosis Regulatory Proteins pharmacology
  • Autophagy
  • Caspase 3 metabolism
  • Caspase 9 metabolism
  • Female
  • Humans
  • Ischemia
  • Kidney pathology
  • Leptin metabolism
  • Leptin pharmacology
  • Male
  • Mammals metabolism
  • Mice
  • Proto-Oncogene Proteins c-akt metabolism
  • Reperfusion adverse effects
  • TOR Serine-Threonine Kinases metabolism
  • Acute Kidney Injury etiology
  • Acute Kidney Injury metabolism
  • Acute Kidney Injury pathology
  • Reperfusion Injury metabolism
Sonstiges:
  • Nachgewiesen in: MEDLINE
  • Sprachen: English
  • Transliterated Title: 瘦素通过抑制细胞凋亡和自噬减轻急性缺血再灌注引起的肾损伤.
  • Publication Type: Journal Article
  • Language: English; Chinese
  • [Zhong Nan Da Xue Xue Bao Yi Xue Ban] 2022 Jan 28; Vol. 47 (1), pp. 8-17.
  • MeSH Terms: Acute Kidney Injury* / etiology ; Acute Kidney Injury* / metabolism ; Acute Kidney Injury* / pathology ; Reperfusion Injury* / metabolism ; AMP-Activated Protein Kinases / metabolism ; Animals ; Apoptosis ; Apoptosis Regulatory Proteins / metabolism ; Apoptosis Regulatory Proteins / pharmacology ; Autophagy ; Caspase 3 / metabolism ; Caspase 9 / metabolism ; Female ; Humans ; Ischemia ; Kidney / pathology ; Leptin / metabolism ; Leptin / pharmacology ; Male ; Mammals / metabolism ; Mice ; Proto-Oncogene Proteins c-akt / metabolism ; Reperfusion / adverse effects ; TOR Serine-Threonine Kinases / metabolism
  • References: Eur J Pharmacol. 2012 Dec 5;696(1-3):143-54. (PMID: 23022334) ; Cell Cycle. 2011 Sep 1;10(17):2917-23. (PMID: 21857156) ; Genet Mol Res. 2015 Dec 21;14(4):17373-83. (PMID: 26782378) ; Transplantation. 2013 Mar 15;95(5):653-7. (PMID: 23503499) ; Crit Care. 2016 Jul 04;20(1):188. (PMID: 27373891) ; J Transl Med. 2013 Jul 11;11:170. (PMID: 23841921) ; Transplantation. 2007 Nov 15;84(9):1183-90. (PMID: 17998875) ; Int Immunopharmacol. 2021 Jul;96:107794. (PMID: 34162156) ; Am J Physiol Renal Physiol. 2012 Dec 1;303(11):F1487-94. (PMID: 22993069) ; Gynecol Oncol. 2021 Oct;163(1):191-198. (PMID: 34400005) ; Bratisl Lek Listy. 2017;118(8):443-448. (PMID: 29050480) ; Am J Pathol. 2010 Mar;176(3):1181-92. (PMID: 20075199) ; PLoS One. 2018 Jan 2;13(1):e0190765. (PMID: 29293685) ; Am J Physiol Heart Circ Physiol. 2010 Oct;299(4):H1265-70. (PMID: 20656889) ; FEBS J. 2008 Jun;275(12):3136-44. (PMID: 18479463) ; Kidney Int. 2012 Dec;82(12):1271-83. (PMID: 22854643) ; Compr Physiol. 2017 Dec 12;8(1):351-369. (PMID: 29357132) ; Clin J Am Soc Nephrol. 2013 Sep;8(9):1482-93. (PMID: 23744003) ; Kidney Int. 2013 Sep;84(3):457-67. (PMID: 23636171) ; PLoS One. 2014 Jun 12;9(6):e99187. (PMID: 24922063) ; Lancet. 2019 Nov 23;394(10212):1949-1964. (PMID: 31777389) ; Biochem Cell Biol. 2018 Jun;96(3):349-354. (PMID: 28544853) ; Front Immunol. 2021 Jul 26;12:697751. (PMID: 34381450)
  • Grant Information: 81770692 the National Natural Science Foundation of China
  • Contributed Indexing: Keywords: acute kidney injury; apoptosis; autophagy; ischemia/reperfusion; leptin ; Local Abstract: [Publisher, Chinese] 目的 : 急性肾损伤(acute kidney injury,AKI)可由缺血再灌注(ischemia/reperfusion,I/R)、肾毒素和败血症等引起,预后差,病死率高。瘦素(leptin)是一种蛋白质分子,主要通过与其特异性受体结合来调节机体能量代谢和生殖活动。Leptin可抑制I/R损伤导致的心肌细胞凋亡,但其对I/R肾损伤的影响及其机制尚不明确。本研究旨在探讨leptin在急性I/R肾损伤过程中对肾功能、肾组织病理、细胞凋亡和自噬的影响及其机制。 方法 : 将健康成年雄性小鼠随机分为4组:假手术(sham)+野生型小鼠(ob/+)组、sham+leptin基因缺陷型小鼠(ob/ob)组、I/R+ob/+组、I/R+ob/ob组,每组8只。假手术处理为在小鼠背部做纵向切口,暴露、分离双侧肾及肾动脉,不作后续处理。I/R处理为缺血30 min,再灌注48 h。检测BUN和SCr水平以评价肾功能;采用HE染色观察肾组织病理变化;采用TUNEL染色观察细胞凋亡,计数凋亡阳性细胞;采用蛋白质印迹法检测小鼠凋亡相关蛋白质(caspase 3、caspase 9),自噬相关蛋白质[哺乳动物雷帕霉素靶蛋白(mammalian target of rapamycin,mTOR)、磷酸化的mTOR(p-mTOR)、LC3 I、LC3 II],mTOR依赖的信号通路蛋白质[磷酸酯酶与张力蛋白同源物(phosphate and tension homology,PTEN)、腺苷单磷酸活化蛋白激酶(adenosine monophosphate-activated protein kinase,AMPK)、蛋白激酶B(protein kinase B,AKT)、细胞外调节蛋白激酶(extracellular regulated protein kinase,ERK)、磷酸化的PTEN(p-PTEN)、磷酸化的AMPK(p-AMPK)、磷酸化的AKT(p-AKT)、磷酸化的ERK(p-ERK)]的表达水平。 结果 : Sham+ob/+组与sham+ob/ob组小鼠的BUN和SCr水平差异均无统计学意义(均 P >0.05)。I/R+ob/+组小鼠的BUN和SCr水平较sham+ob/+组小鼠均显著上升(均 P <0.05),I/R+ob/ob组小鼠的BUN和SCr水平较sham+ob/ob组和I/R+ob/+组小鼠均显著上升(均 P <0.05)。Sham+ob/+组与sham+ob/ob组小鼠肾小管无明显损伤。与sham+ob/+组和sham+ob/ob组相比,I/R+ob/+组和I/R+ob/ob组均出现肾小管上皮细胞刷状缘脱落、空泡变性和蛋白管型形成等细胞损伤表现。与I/R+ob/+组相比,I/R+ob/ob组小鼠肾小管受损更严重。肾小管损伤病理评分结果显示I/R+ob/ob组小鼠肾小管损伤最严重( P <0.05)。与sham+ob/+组相比,I/R+ob/+组的caspase 3、caspase 9、PTEN和LC3 II蛋白质水平明显上调,LC3 II/LC3 I比值明显升高,p-mTOR、p-PTEN、p-AMPK、p-AKT和p-ERK蛋白质表达水平明显下调(均 P <0.05);与sham+ob/ob组相比,I/R+ob/ob组的caspase 3、caspase 9、PTEN和LC3 II蛋白质表达水平明显上调,LC3 II/LC3 I比值明显升高,而p-mTOR、p-PTEN、p-AMPK、p-AKT和p-ERK蛋白质表达水平明显下调(均 P <0.05);且与I/R+ob/+组相比,I/R+ob/ob组的p-mTOR、p-PTEN、p-AMPK、p-AKT和p-ERK蛋白质表达水平下调更明显,caspase 3、caspase 9、PTEN、LC3 II蛋白质表达水平上调更明显,LC3 II/LC3 I比值升高更明显(均 P <0.05)。 结论 : 小鼠肾急性I/R后出现肾功能和肾小管损伤,凋亡和自噬水平升高。Leptin可能通过抑制凋亡和mTOR依赖的信号通路相互作用构成的复杂网络调控自噬减轻肾急性 I/R损伤。.
  • Substance Nomenclature: 0 (Apoptosis Regulatory Proteins) ; 0 (Leptin) ; EC 2.7.11.1 (Proto-Oncogene Proteins c-akt) ; EC 2.7.11.1 (TOR Serine-Threonine Kinases) ; EC 2.7.11.31 (AMP-Activated Protein Kinases) ; EC 3.4.22.- (Caspase 3) ; EC 3.4.22.- (Caspase 9)
  • Entry Date(s): Date Created: 20220511 Date Completed: 20220516 Latest Revision: 20240321
  • Update Code: 20240321
  • PubMed Central ID: PMC10930488

Klicken Sie ein Format an und speichern Sie dann die Daten oder geben Sie eine Empfänger-Adresse ein und lassen Sie sich per Email zusenden.

oder
oder

Wählen Sie das für Sie passende Zitationsformat und kopieren Sie es dann in die Zwischenablage, lassen es sich per Mail zusenden oder speichern es als PDF-Datei.

oder
oder

Bitte prüfen Sie, ob die Zitation formal korrekt ist, bevor Sie sie in einer Arbeit verwenden. Benutzen Sie gegebenenfalls den "Exportieren"-Dialog, wenn Sie ein Literaturverwaltungsprogramm verwenden und die Zitat-Angaben selbst formatieren wollen.

xs 0 - 576
sm 576 - 768
md 768 - 992
lg 992 - 1200
xl 1200 - 1366
xxl 1366 -