N^6-(6-氨基己基)-5′-磷酸腺苷的合成(英文)

由肌苷开始经五步合成出Ｎ６－（６－氮基己基）－５’－磷酸腺苷。对６－氯－９β－Ｄ－呋喃核糖嘌呤的合成进行了改进。１，６－己二胺同６－氯－９β－Ｄ呋喃核糖嘌呤－５’－磷酸发生取代反应，合成出Ｎ６－（６－氮基己基）－５′－磷酸腺苷，基于核苷的总产率约７０％。

β-细辛醚对肾癌增殖及迁移侵袭的影响及其分子机制

目的研究β-细辛醚(β-As)对肾癌细胞的抑制作用及其分子机制,帮助阐明β-As抗肾肿瘤的作用并为其临床转化提供参考。方法本实验选用人肾癌细胞786-O和769-P进行体外实验,使用小鼠肾癌细胞Renca进行体内实验。应用MTT法、细胞划痕试验、细胞侵袭实验(Transwell)小室检测肾癌细胞体外增殖、迁移侵袭能力;应用蛋白印迹法检测自噬及上皮间质转化(EMT)等相关蛋白水平的变化;应用Balb/c小鼠皮下成瘤实验检测β-As在体内的抗肿瘤作用。结果β-As可通过剂量依赖的方式抑制肾癌细胞786-O和769-P体外增殖。β-As可上调E-cadherin的表达,下调N-cadherin、Vimentin的表达,并抑制其体外迁移侵袭能力。β-As可通过剂量依赖的方式上调LC3-Ⅱ、p-AMPK表达,下调p-mTOR、p-S6K的表达,而对总的AMPK、mTOR表达水平无显著影响。体内实验发现β-As可抑制肾癌细胞增殖。结论β-细辛醚通过自噬依赖性AMPK/mTOR信号通路对肾癌细胞的生长增殖、迁移侵袭及EMT进行抑制,在肾透明细胞癌尤其是进展期肾癌方面具有一定的临床转化潜能。

HSF1/AMPK信号通路在铁死亡参与糖尿病心肌病发病的机制研究

目的:探讨热休克因子1(heat shock factor 1,HSF1)/5′-单磷酸腺苷活化蛋白激酶(adenosine monophosphate activated protein kinase,AMPK)信号通路调控铁死亡对糖尿病心肌病(diabetic cardiomyopathy,DCM)发病的影响。方法:本研究为实验研究,采用空白对照与多组实验对照。H9c2细胞随机分为4组:低葡萄糖组(control,Con)、高葡萄糖组(high glucose,HG)、HG+HSF1组、HG+HSF1+化合物C(compound C,CC)组。分别对细胞进行罗丹明胶质蛋白染色、细胞线粒体(reactive oxygen species,ROS)检测和细胞脂质ROS检测,并通过Western blot分析AMPK信号表达。雄性C57/BL6小鼠随机分为4组:NC组、NC+HSF1组、DM组和DM+HSF1组,每组12只。通过超声心动图评估了小鼠心血管功能参数。结果:与Con组相比,HG组HSF1、pAMPK/AMPK水平明显下调(P=0.005、0.002),和相对细胞表面积、线粒体Fe2+水平、线粒体ROS水平、细胞脂质ROS水平明显增加(P=0.001、0.003、0.006、0.002)。与HG组相比,HG+HSF1组明显逆转了这些变化(P=0.001、0.001、0.002、0.006、0.007、0.003),但加入CC时HSF1的逆转作用明显减弱(P<0.05)。与NC组相比,DM组EF%、FS%、E/A、E′/A′和心脏组织中HSF1、pAMPK/AMPK表达明显降低(均P<0.01),和心脏组织中Fe2+、ROS、丙二醛(Malondialdehyde,MDA)水平和4-羟基壬烯酸(4-Hydroxynonenal,4-HNE)蛋白水平明显增加(P=0.004、0.003、0.001、0.004),DM+HSF1组明显逆转了这些变化。结论:HSF1在DCM病理过程中发挥心脏保护作用,其抗铁死亡作用可能与AMPK依赖性的脂质代谢和线粒体稳态调节有关。

阿司匹林调控肿瘤细胞自噬机制的研究进展

阿司匹林可通过多种信号通路调节细胞自噬而发挥其抗肿瘤作用。文章主要就阿司匹林通过AMPK依赖性和非依赖性途径诱导肿瘤细胞自噬的分子机制进行综述,为深入理解阿司匹林的防癌抗癌机制提供参考。

二甲双胍通过AMPK-自噬信号通路促进脑保护作用的研究

目的 探讨二甲双胍(Met)预处理能否对心搏骤停/心肺复苏(CA/CPR)后脑损伤起到保护作用及其可能的机制及信号通路。方法 以电刺激法构建CA模型。将大鼠随机分为假手术组(0.9%NaCl灌胃14 d,不诱导CA)、模型组(0.9%NaCl灌胃14 d后造模)、实验组(200 mg·kg^(-1)Met+0.9%NaCl灌胃14 d后造模)、Cc组[200 mg·kg^(-1)Met+0.9%NaCl灌胃14 d,造模前1 h经腹膜腔注射5′-腺嘌呤核苷酸依赖的蛋白激酶(AMPK)抑制药Cc]、氯喹组[200 mg·kg^(-1)Met+0.9%NaCl灌胃14 d,造模前1 h腹膜腔注射自噬抑制药氯喹]和AICAR组(200 mg·kg^(-1)Met+0.9%NaCl灌胃14 d,造模前1 h经腹膜腔注射AMPK激动药AICAR)。以生存曲线记录CA/CPR后7 d生存率,以神经病残疾评分表对CA/CPR后7 d神经功能进行评分,以考马斯亮蓝法测定丙二醛(MDA)水平;以活性氧簇(ROS)荧光探针DHE检测脑组织ROS水平,以蛋白质印迹法测定脑组织中AMPK、p-AMPK、微管相关蛋白轻链3Ⅰ(LC3Ⅰ)、LC3Ⅱ、p62蛋白表达水平。结果 假手术组、模型组、实验组、Cc组、氯喹组、AICAR组大鼠的7 d生存率分别100%、40%、70%、40%、40%和65%,7 d神经功能评分分别为(78.35±1.65)、(46.50±4.41)、(67.93±4.64)、(49.50±3.53)、(52.00±2.83)和(68.33±1.53)分,ROS水平分别为(417.60±8.37)、(748.60±36.05)、(575.80±10.73)、(713.80±18.85)、(668.20±9.58)和(566.00±24.48)U·mg^(-1),MDA水平分别为(4.38±0.33)、(8.06±0.76)、(5.50±0.48)、(7.18±0.29)、(6.82±0.31)和(5.20±0.34)nmol·mg^(-1),p-AMPK/AMPK水平分别为0.74±0.04、0.87±0.01、1.61±0.01、0.55±0.05、1.09±0.09和1.27±0.07,p62相对表达水平分别为0.42±0.02、0.86±0.05、0.61±0.04、0.98±0.04和0.78±0.03,LC3Ⅱ/LC3Ⅰ水平分别为0.29±0.32、0.37±0.26、0.96±0.78、0.58±0.26、0.43±0.03和1.40±0.10。实验组、AICAR组的上述指标与模型组比较,Cc组、氯喹组的上述指标与实验组比较,差异均有统计学意义(均P<0.05)。结论 Met预处理通过激活AMPK信号通路、调节线粒体能量代谢、促进自噬而对大鼠CA/CPR后脑损伤发挥保护作用。

罗格列酮促进AMPK蛋白磷酸化改善db/db小鼠胰岛素抵抗

【目的】观察罗格列酮对2型糖尿病db/db小鼠肝脏、骨骼肌和脂肪中5′-单磷酸腺苷活化蛋白激酶(AMPK)和葡萄糖转运蛋白4(GLUT4)的蛋白表达的影响,了解罗格列酮调节AMPK信号通路的初步机制。【方法】将db/db小鼠按血糖浓度随机分层分为模型组和罗格列酮组;同窝出生的db/m小鼠为正常对照组。灌胃给药4周(罗格列酮5 mg/kg,其余组给予同等剂量的生理盐水),分别于用药2周和4周后检测小鼠的空腹血糖;用药4周末处死动物,立即取肝脏、皮下脂肪组织和腓肠肌,置于-80℃环境保存,用免疫印迹试验(Western blot)检测AMPK、p-AMPK以及GLUT4的蛋白表达。【结果】①罗格列酮显著降低db/db小鼠的空腹血糖浓度。用药2周后模型组血糖浓度为(22.09±3.67)mmol/L,罗格列酮组血糖浓度为(14.18±3.59)mmol/L(P<0.05);用药4周后模型组血糖浓度为(23.08±3.66)mmol/L,罗格列酮组血糖浓度为(14.18±3.59)mmol/L(P<0.01);②罗格列酮可上调db/db小鼠肝脏、骨骼肌和脂肪组织AMPK磷酸化水平,增加骨骼肌和脂肪组织的GLUT4蛋白含量。【结论】罗格列酮可增加db/db小鼠肝脏、肌肉和脂肪组织AMPK的磷酸化和GLUT4的蛋白表达,促进外周组织的葡萄糖摄取和利用,提示其可部分通过AMPK通路调节db/db小鼠的糖代谢。

枸杞多糖调控AMPK/Sirt自噬途径延缓D-gal诱导的卵巢早衰的机制研究

从5′-单磷酸腺苷活化蛋白激酶(5′-adenosine monophosphate activated protein kinase, AMPK)/沉默信息调节因子1(silent information regulator 1,Sirt1)信号通路,探讨枸杞多糖缓解小鼠卵巢早衰(POF)的分子机制。采用背部注射D-半乳糖(D-gal)法建立POF小鼠模型,实验设置正常对照组、模型组、枸杞多糖组、3-MA组(自噬抑制剂3-甲基腺嘌呤)、AMPK抑制剂组、枸杞多糖+AMPK抑制剂组,每组15只,各组连续给药28 d后;酶联免疫吸附测定(enzyme-linked immunosorbent assay, ELISA)法检测血清性激素[雌二醇(estradiol, E2)、黄体生成激素(luteinizing hormone, LH)、卵泡刺激素(follicle-stimulating hormone, FSH)]水平;检测卵巢质量系数;SA-β-Gal苷酶染色观察卵巢衰老状态;苏木素-伊红(hematoxylin-eosin, HE)染色观察卵巢形态变化;免疫组化法检测自噬标记物-LC3-Ⅱ在卵巢组织中表达;蛋白免疫印迹(Western blot)法检测衰老标记因子-p16INK4a、自噬标记物LC3-Ⅱ、Beclin-1、自噬底物p62、溶酶体相关膜蛋白2(LAMP2)、自噬调控通路AMPK/Sirt1/雷帕霉素靶蛋白复合体1(mTORC1)/Unc-51样激酶1 Ser757位点(Ulk1 Ser757)蛋白表达。与正常对照组相比,模型组小鼠卵巢颗粒细胞及各级卵泡减少严重,卵巢组织衰老及性激素分泌紊乱严重,卵巢自噬活性减弱,AMPK/Sirt1自噬途径蛋白表达降低(P<0.05)。枸杞多糖干预治疗后,小鼠卵巢颗粒细胞及各级卵泡减少、衰老及性激素紊乱现象减轻,自噬活性升高,AMPK/Sirt1自噬途径活化(P<0.05)。3-MA及AMPK抑制剂干预治疗,均可抑制自噬,加重小鼠卵巢损伤及衰老,AMPK抑制剂可部分减弱枸杞多糖发挥的促进自噬活化、抗衰老及改善卵巢组织损伤作用(P<0.05)。枸杞多糖可通过促进AMPK/Sirt1自噬途径活化,来缓解D-gal诱导的POF症状。

Study on the relationship between relieving energy crisis in myofascial trigger points with An-Pressing manipulation and AMPK/PGC-1α pathway activation

Objective To explore the mechanism of An-Pressing manipulation in relieving energy crisis in chronic myofascial trigger points(MTrPs)by observing the effects of An-Pressing manipulation on adenosine triphosphate(ATP),adenosine 5′-monophosphate(AMP)-activated protein kinase(AMPK)/peroxisome proliferator-activated receptorγcoactivator 1α(PGC-1α)pathway and mitochondrial ultrastructure of skeletal muscle cells in MTrPs rats.Methods Forty-eight male Sprague-Dawley rats were randomly divided into a blank group,a model group,a lidocaine group,and an An-Pressing manipulation group,with 12 rats in each group.The model group,lidocaine group and An-Pressing manipulation group were used to replicate the MTrPs rat model by blunt shock and centrifugal motion method.After modeling,the An-Pressing manipulation group was subjected to 7 times An-Pressing manipulation,once every other day;the lidocaine group was treated with 3 times of injection of lidocaine at the MTrPs,once every 6 d.The blank group and the model group were fed normally without intervention.After the intervention,local muscle tissue was taken to detect the content of ATP and the expression of AMPK,phosphorylated AMPK(phospho-AMPK),PGC-1α,and glucose transporter 4(GluT4),and the ultrastructure of mitochondria was observed under an electron microscope.Results Compared with the blank group,the ATP content in the model group was decreased(P<0.05),the protein expression levels of phospho-AMPK,PGC-1α,and GluT4 and the ratio of phospho-AMPK to AMPK were decreased(P<0.05);under the electron microscope,the number of mitochondria decreased,and they were deformed,small in volume,and had deformed cristae.Compared with the model group,the ATP contents in the An-Pressing manipulation group and the lidocaine group were increased(P<0.05),and the protein expression levels of phospho-AMPK,PGC-1α,and GluT4 and the ratio of phospho-AMPK to AMPK were increased(P<0.05);under the electron microscope,the number of mitochondria increased,the shape and size of the mitochondria were basically normal,and the cristae could be seen.Compared with the lidocaine group,phospho-AMPK and the ratio of phospho-AMPK to AMPK in the An-Pressing manipulation group were increased(P<0.05);under the electron microscope,the numbers of mitochondria were similar,and the shape and size of the mitochondria were basically normal without swelling,and the cristae could be observed.Conclusion An-Pressing manipulation can increase the ATP content in MTrPs tissue,improve the expression levels of PGC-1α and GluT4 proteins and the ratio of phospho-AMPK to AMPK;its mechanism may relate to the activation of AMPK/PGC-1α signaling pathway to promote the repair of mitochondrial damages.