Effect of Amygdalin on the Proliferation of Hyperoxia-exposed Type Ⅱ Alveolar Epithelial Cells Isolated from Premature Rat

Summary: The pathogenesis of hyperoxia lung injury and the mechanism of amygdalin on type 2 alveolar epithelial cells (AEC2) isolated from premature rat lungs in vitro were investigated. AEC2 were obtained by primary culture from 20-days fetal rat lung and hyperoxia-exposed cell model was established. Cell proliferating viability was examined by MTT assay after treatment of amygdalin at various concentrations. DNA content and the proliferating cell nuclear antigen (PCNA) protein expression of AEC2 were measured by using flow cytometry and immunocytochemistry respectively after 24 h of hyperoxia exposure or amygdalin treatment. The results showed that hyperoxia inhibited the proliferation and decreased PCNA protein expression in AEC2 of premature rat in vitro. Amygdalin at the concentration range of 50-200 μmol/L stimulated the proliferation of AEC2 in a dose-dependent manner, however, 400 μmol/L amygdalin inhibited the proliferation of AEC2. Amygdalin at the concentration of 200 μmol/L played its best role in facilitating proliferation of AEC2s in vitro and could partially ameliorated the changes of proliferation in hyperoxia exposed AEC2 of premature rat. It has been suggested that hyperoxia inhibited the proliferation of AEC2s of premature rat, which may contribute to hyperoxia lung injury. Amygdalin may play partial protective role in hyperoxia-induced lung injury.

Primary Culture of Alveolar Epithelial Type Ⅱ Cells and Its Bionomic Study

To establish a better method of primary culture for alveolar epithelial type Ⅱ cells （AEC Ⅱ ） and to study its bionomics, alveolar epithelial type Ⅱ cells were isolated by digestion with trypsin and collagenase, which were then purified by plated into culture flask coated with rat immunoglobulin （i The purified AEC Ⅱ were identified by alkaline phosphatase staining, electron mi- croscopy, immunocytochemical staining of pulmonary surfactant protein A （SPA）. The SPA expression and transfection characteristics were compared with those of A549 cell line. The results showed that AEC Ⅱ could be isolated by digestion with trysin and collagenase and purified by adhesive purification by using IgG, with a yield of about 2-3 × 10^7, and a purity of about 75%-84 %. Cells could be quickly identified with AKP staining. AEC Ⅱ were different from A549 cell line in terms of SPA expression and transfection characteristics. It is concluded that adhesive purification with IgG can improve the purity of AEC Ⅱ, and AKP staining is simple in cell identification. AEC Ⅱ can not be completely replaced by A549 cells in some studies because the differences between them, such as SPA expression.

Effects of Hyperoxia on Cytoplasmic Thioredoxin System in Alveolar Type Epithelial Cells of Premature Rats

This study investigated the effects of hyperoxia on dynamic changes of thioredoxin-1 （Trx1） and thioredoxin reductase-1 （TrxR1） in alveolar type Ⅱ epithelial cells （AECⅡ） of premature rats. Pregnant Sprague-Dawley rats were sacrificed on day 19 of gestation. AECⅡ were isolated and purified from the lungs of premature rats. When cultured to 80% confluence, in vitro cells were randomly divided into air group and hyperoxia group. Cells in the hyperoxia group were continuously exposed to 95% O2/5% CO2 and those in the air group to 95% air/5% CO2. After 12, 24 and 48 h, cells in the two groups were harvested to detect their reactive oxygen species （ROS）, apoptosis, TrxR1 activity and the expressions of Trx1 and TrxR1 by corresponding protocols, respectively. The results showed that AECⅡ exposed to hyperoxia generated excessive ROS and the apoptosis percentage in the hyperoxia group was increased significantly at each time points as compared with that in the air group （P0.001）. Moreover, TrxR1 activity was found to be markedly depressed in the hyperoxia group in comparison to that in the air group （P0.001）. RT-PCR showed the expressions of both Trx1 and TrxR1 mRNA were significantly increased in AECⅡ exposed to hyperoxia for 12 and 24 h （P0.01）, respectively. At 48 h, the level of Trx1 mRNA as well as that of TrxR1 mRNA in the hyperoxia group was reduced and showed no significant difference from that in the air group （P0.05）. Western blotting showed the changes of Trx1 protein expressions in the hyperoxia group paralleled those of Trx1 mRNA expressions revealed by RT-PCR. It was concluded that hyperoxia can up-regulate the protective Trx1/TrxR1 expressed by AECⅡ in a certain period, however, also cause dysfunction of the cytoplasmic thioredoxin system by decreasing TrxR1 activity, which may contribute to the progression of oxidative stress and cell apoptosis and finally result in lung injury.

Role of mechanical stretching and lipopolysaccharide in early apoptosis and IL-8 of alveolar epithelial typeⅡcells A549

Objective:To investigate the effects of mechanical stretching and lipopolysaccharide(LPS) on the early apoptosis and IL-8 production of alveolar epithelial type II cells A549.Methods:The experimental matrix consisted of three integrated studies.In the first study,A549 cells were subjected to different stretching strain frequency and duration time to see the effects on the early apoptosis.In the second study,A549 cells were subjected to mechanical stretch(13%4 h, 0.3 Hz) and LPS(1 or 100 ng/mL) to see whether mechanical strain and LPS also have an addictive effect on the early apoptosis.In the third study to investigate whether this addictive effect could be induced by LPS and mechanical stretch on IL-8 production,A549 cells were subjected to LPS(100 ng/mL) and mechanical strain(13%.0.3 Hz,4 h).Real time PCR and enzyme linked immunosorbent assay were used to measure mRN A and protein level of IL-8.The early apoptosis was detected by flow cytometry.Results:Mechanical stretch induced the early apoptosis in a force and frequency and time-dependent manner.In the presence of LPS,mechanical stretch enhanced LPS-induced early apoptosis,especially in 100 ng/mL IPS group compared with 1 ng/ mL LPS and the control group.Mechanical stretch increased IL-8 production and enhanced LPS-induced IL-8 screation both in mRNA and protein levels.Conclusions:Mechanical stretch can induce the early apoptosis and IL-8 secretion.Mechanical stretch and LPS have an addictive effect on the early apoptosis and IL-8 production in alveolar type 2 cells,which is one of the mechanisms of ventilator-induced lung injury.

Hypoxia upregulates hypoxia inducible factor(HIF)-3α expression in lung epithelial cells: characterization and comparison with HIF-1α

The role of the hypoxia-inducible factor(HIF)subunits 1α and 2α in response to hypoxia is well established in lungepithelial cells,whereas little is known about HIF-3α with respect to transcriptional and translational regulation by hy-poxia.HIF-3α and HIF-1α are two similar but distinct basic helix-loop-helix-PAS proteins,which have been postulatedto activate hypoxia responsive genes in response to hypoxia.Here,we used quantitative real time RT-PCR and immu-noblotting to determine the activation of HIF-3α vs.HIF-1α by hypoxia.HIF-3α was strongly induced by hypoxia(1%O_2)both at the level of protein and mRNA due to an increase in protein stability and transcriptional activation,whereasHIF-1α protein and mRNA levels enhanced transiently and then decreased because of a reduction in its mRNA stabilityin A549 cells,as measured on mRNA and protein levels.Interestingly,HIF-3α and HIF-1α exhibited strikingly similarresponses to a variety of activating or inhibitory pharmacological agents.These results demonstrate that HIF-3α is ex-pressed abundantly in lung epithelial cells,and that the transcriptional induction of HIF-3α plays an important role in theresponse to hypoxia in vitro.Our findings suggest that HIF-3α,as a member of the HIF system,is complementary ratherthan redundant to HIF-1α induction in protection against hypoxic damage in alveolar epithelial cells.

Deletion of SMARCA4 impairs alveolar epithelial type II cells proliferation and aggravates pulmonary fibrosis in mice

Alveolar epithelial cells(AECs)injury and failed reconstitution of the AECs barrier are both integral to alveolar flooding and subsequent pulmonary fibrosis(PF).Nevertheless,the exact mechanisms regulating the regeneration of AECs post-injury still remain unclear.SMARCA4 is a part of the large ATP-dependent chromatin remodelling complex SWI/SNF,which is essential for kidney and heart fibrosis.We investigates SMARCA4 function in lung fibrosis by establishing PF mice model with bleomycin firstly and found that the expression of SMARCA4 was mainly enhanced in alveolar type II(ATII)cells.Moreover,we established an alveolar epithelium-specific SMARCA4-deleted SP-C-rtTA/(tetO)7-Cre/SMARCA4f/f mice(SOSM4D/D)model,as well as a new SMARCA4-deleted alveolar type II(ATII)-like mle-12 cell line.We found that the bleomycin-induced PF was more aggressive in SOSM4D/D mice.Also,the proliferation of ATII cells was decreased with the loss of SMARCA4 in vivo and in vitro.In addition,we observed increased proliferation of ATII cells accompanied by abnormally high expression of SMARCA4 in human PF lung sections.These data uncovered the indispensable role of SMARCA4 in the proliferation of ATII cells,which might affect the progression of PF.

Continuous purification and culture of rat type 1 and type 2 alveolar epithelial cells by magnetic cell sorting

Purpose:The incidence of acute lung injury(ALI)in severe trauma patients is 48%and the mortality rate following acute respiratory distress syndrome evolved from ALI is up to 68.5%.Alveolar epithelial type 1 cells(AEC1 s)and type 2 cells(AEC2s)are the key cells in the repair of injured lungs as well as fetal lung development.Therefore,the purification and culture of AECls and AEC2s play an important role in the research of repair and regeneration of lung tissue.Methods:Sprague-Dawley rats(3-4 weeks,120-150 g)were purchased for experiment.Dispase and DNase I were jointly used to digest lung tissue to obtain a single-cell suspension of whole lung cells,and then magnetic bead cell sorting was performed to isolate Tla positive cells as AECls from the single-cell suspension by using polyclonal rabbit anti-Tla(a specific AECls membrane protein)antibodies combined with anti-rabbit IgG microbeads.Afterwards,alveolar epithelial cell membrane marker protein EpCAM was designed as a key label to sort AEC2s from the remaining Tla-neg cells by another positive immunomagnetic selection using monoclonal mouse anti-EpCAM antibodies and anti-mouse IgG microbeads.Cell purity was identified by immunofluorescence staining and flow cytometry.Resii沾••The purity of AECls and AEC2s was 88.3%±3.8%and 92.6%±2.7%,respectively.The cell growth was observed as follows:AECls stretched within the 12-16 h,but the cells proliferated slowly;while AEC2s began to stretch after 24 h and proliferated rapidly from the 2nd day and began to differentiate after 3 days.Conclusion:AECls and AEC2s sorted by this method have high purity and good viability.Therefore,our method provides a new approach for the isolation and culture of AECls and AEC2s as well as a new strategy for the research of lung repair and regeneration.

类视黄醇X受体对缺氧/复氧诱导的大鼠Ⅱ型肺泡上皮细胞氧化应激反应的调控作用

目的:探讨类视黄醇X受体(RXR)在缺氧/复氧(HR)诱导的大鼠Ⅱ型肺泡上皮细胞(AECⅡ)氧化应激反应中的调控作用。方法:随机将细胞实验分成5组:对照(C)组、HR组、HR+溶剂二甲基亚砜(DMSO)组(HD组)、HR+RXR激动剂9-顺式维甲酸(9-RA)组(RA组)和HR+RXR抑制剂HX531组(HX组)。采用CCK-8法检测各组细胞活力;免疫荧光法进行AECⅡ特异性指标表面活性物质蛋白A(SP-A)的鉴定和RXRα表达的观察;试剂盒检测细胞内超氧化物歧化酶(SOD)活性和丙二醛(MDA)含量;透射电镜观察细胞内超微结构的变化;Western blot检测核因子E2相关因子2(Nrf2)蛋白水平;RT-PCR检测Nrf2的mRNA表达水平。结果:与C组相比,HR、HD、RA和HX组细胞活力均显著降低(P<0.05),SOD活性显著下降(P<0.05),MDA含量显著增高(P<0.05),Nrf2的mRNA和蛋白表达水平显著降低(P<0.05或P<0.01),RXRα的免疫荧光表达显著增加(P<0.01);与HR和HX组相比,RA组细胞活力增加(P<0.05),SOD活性上升(P<0.05),MDA含量下降(P<0.05),Nrf2的mRNA和蛋白表达水平升高(P<0.01),RXRα的免疫荧光表达显著增加(P<0.01)。结论:HR可加剧大鼠AECⅡ的氧化应激反应,RXR激动剂干预后可通过抑制氧化应激反应减轻HR引起的大鼠AECⅡ损伤。

大鼠Ⅰ型肺泡上皮细胞的分离、培养及生物学特性研究

目的改良细胞分离方法,得到高纯度的原代Ⅰ型肺泡上皮细胞(ATⅠ)并进行培养,初步观察其生物学特性。方法采用SPF级SD大鼠,通过酶消化法、IgG贴壁法和免疫磁珠法获得高纯度ATⅠ并进行培养,采用台盼蓝染色计算细胞活力,免疫荧光DAPI法鉴定细胞纯度和表型,倒置显微镜观察细胞生长规律,计数法绘制细胞生长曲线。结果每只体重120g左右的SD大鼠可获得(2.1±0.5)×106个ATⅠ,细胞活力为93.8%±1.6%,细胞纯度为91.0%±0.6%。培养3d后细胞完全黏附、伸展,培养7d后汇合形成单层扁平状。免疫荧光检测显示,培养的原代细胞水通道蛋白5(AQP5)和小窝蛋白1(Cav-1)呈阳性表达,表面活性蛋白C前体(pro-SPC)呈阴性表达。获取的ATⅠ可在体外增殖,生长曲线显示原代ATⅠ在对数增长期的倍增时间约为66h。结论改良细胞分离方法可以得到高纯度的ATⅠ,培养后细胞生长良好,可为研究以ATⅠ损伤为特征的肺部疾病提供可靠的体外模型。

曲格列酮对转化生长因子-β_1诱导的HK-2细胞纤连蛋白和胶原Ⅰ型基因表达的影响

目的观察曲格列酮对转化生长因子-β1(TGF-β1)诱导的人肾近曲小管上皮细胞(HK-2)细胞外基质纤连蛋白和胶原Ⅰ型的影响,探讨曲格列酮抗肾间质纤维化的潜在作用。方法将曲格列酮0,0.25,0.5,1,2.5,5和10μmol.L-1预处理HK-2细胞2h,随后加入TGF-β15mg.L-1作用24h,利用乳酸脱氢酶(LDH)释放实验检测曲格列酮对HK-2细胞的毒性作用;曲格列酮0,1,2.5,5和10μmol.L-1预处理HK-2细胞2h,再加入TGF-β15mg.L-1作用24h,通过实时荧光定量PCR检测HK-2细胞外基质主要成分胶原Ⅰ型mRNA和纤连蛋白mRNA表达。结果曲格列酮0.25～5μmol.L-1对HK-2细胞膜完整性无影响,LDH的释放与正常对照组无明显差异,曲格列酮10μmol.L-1组LDH释放率为(10.7±5.3)%,明显高于正常对照组(P<0.01)。与正常对照组相比,曲格列酮1,2.5,5和10μmol.L-1单独作用并没有增加HK-2细胞外基质中胶原Ⅰ型纤维和纤连蛋白的表达,而TGF-β1刺激下胶原Ⅰ型纤维和纤连蛋白表达明显上调,曲格列酮提前干预下纤连蛋白mRNA及胶原Ⅰ型mRNA表达下降,曲格列酮2.5,5和10μmo.lL-1可显著下调纤连蛋白mRNA表达(P<0.05,P<0.01);曲格列酮5和10μmol.L-1可显著下调胶原Ⅰ型mRNA表达(P<0.05)。结论曲格列酮可能具有拮抗肾间质纤维化的潜在作用,其作用机制可能与抑制HK-2细胞纤连蛋白和胶原Ⅰ型纤维的增加有关。

miR-146a通过调节IPr1基因对结核分枝杆菌感染的AEC Ⅱ型细胞活性作用机制

目的 探讨miR-146a通过调节IPr1基因观察对结核分枝杆菌(Mtb)感染的肺泡II型上皮细胞(AEC II)活性的作用机制。方法 采用Mtb感染AECⅡ细胞。将AECⅡ细胞分为结核组(感染Mtb)、 NC组(模型+转染miR-146a NC)、转染组(模型+转染miR-146a mimics)。RT-PCR检测AECⅡ细胞miR-146a、Ipr1基因表达;CCK8检测AECⅡ细胞增殖;流式细胞仪检测AECⅡ细胞凋亡;双荧光素酶报告测定Ipr1与miR-146a靶向关系。结果 DIO荧光染色的Mtb在感染人AECⅡ细胞12 h内会进入细胞质基质中,并围绕细胞核分布,表明建立的结核分枝杆菌感染模型成功;结核组与NC组AECⅡ细胞中miR-146a、Ipr1基因表达比较无差异(P>0.05),与NC组相比,转染组AECⅡ细胞中miR-146a、Ipr1基因表达水平升高(P<0.05);结核组与NC组AECⅡ细胞在不同时间点的OD值比较均无差异(P>0.05),与NC组相比,转染组AECⅡ细胞在不同时间点的OD值均升高(P<0.05);结核组AECⅡ细胞凋亡率与NC组相比无差异(P>0.05),与NC组相比,转染组AECⅡ细胞凋亡率显著降低(P<0.001)。双荧光素酶报告结果显示,转染miR-146a后野生型Mtb感染的AECⅡ细胞中Ipr1活性升高(P<0.05),突变型Mtb感染的AECⅡ细胞中Ipr1活性无明显变化(P>0.05),表明Ipr1是miR-146a的靶基因。结论 过表达的miR-146a可增加Mtb感染的AECⅡ细胞活性,降低凋亡,研究机制认为可能与通过激活Ipr1水平相关。Ipr1是miR-146a靶基因,可通过激活表达而发挥减少Mtb对AECⅡ细胞活性的损伤。

中波紫外线和氧化应激诱导LECs中Ⅰ型胶原降解的分子机制研究

目的探讨中波紫外线(UVB)和氧化应激诱导人晶状体上皮细胞(LECs)中Ⅰ型胶原降解的时间和剂量依赖方式及其作用信号通路。方法培养人LECs,用UVB(15mJ/cm2)或H2O2(100μmol/L)分别处理细胞,Western blot法检测不同时间段的Ⅰ型胶原表达和JNK、c-Jun的磷酸化,Glatin酶谱法分析不同时间段的间质胶原酶(MMP-1)表达,且用不同剂量的UVB辐射或不同浓度H2O2作用后检测上述指标。结果在用UVB和H2O2处理后,Ⅰ型胶原的表达明显下降,8h后为0.890,24h后为0.779。UVB和H2O2以时间和剂量依赖的方式诱导JNK-1和c-Jun的磷酸化,MMP-1的表达也以时间依赖的方式增加。结论在人工培养的人LECs中,UVB、H2O2通过时间和剂量的方式诱导JNK和c-Jun的磷酸化,导致MMP-1和Ⅰ型胶原表达,这一作用通路可能形成潜在的治疗后发性白内障的靶点。

重症急性胰腺炎肺损伤发病机制中的肺泡Ⅱ型上皮细胞凋亡的作用及乌司他丁干预的实验研究

目的探讨重症急性胰腺炎(SAP)发病机制中其肺泡Ⅱ型上皮细胞凋亡的作用并对乌司他丁对其干预的作用进行分析。方法将42只健康大鼠随机分为3组,分别为假手术组、模型组与乌司他丁干预组,每组14只,以向大鼠十二指肠乳头内侧胰胆管注射脱氧胆酸钠建立SAP大鼠模型,假手术组大鼠仅打开大鼠腹腔轻轻翻动其胰腺后关闭腹腔,乌司他丁干预组于大鼠建模后给予乌司他丁注射。对几组大鼠术后肺组织及胰腺组织的病理变化及相关指标差异进行分析。结果与假手术组比较,SAP组及乌司他丁干预组TNF⁃α、AMY及MDA水平明显更高,乌司他丁干预组与SAP组比较,TNF⁃α、AMY及MDA水平明显更低(P<0.05)。SAP大鼠伴随着明显的肺损伤状况,假手术组、SAP组、乌司他丁干预组肺湿/干比值分别为3.62±0.56、6.48±0.77、4.69±0.63,血气指标PaCO_(2)、PaO_(2)分别为(31.25±1.03)mmHg、(106.52±2.03)mmHg,(48.67±2.01)mmHg、(73.57±2.44)mmHg和(35.22±1.32)mmHg、(90.22±3.01)mmHg),SAP组及乌司他丁干预组大鼠肺湿/干比值及PaCO_(2)明显上升,PaO_(2)明显下降,相较于SAP组,乌司他丁干预组大鼠的肺湿/干比值及PaCO_(2)更低,PaO_(2)更高(P<0.05)。假手术组大鼠肺泡Ⅱ型上皮细胞凋亡率[(3.58±0.57)%]及Ca^(2+)浓度[(34.52±2.35)%]均显著低于SAP组凋亡率[(29.67±4.52)%]及Ca^(2+)浓度[(82.66±4.66)%]及乌司他丁干预组凋亡率[(14.62±3.67)%]及Ca^(2+)浓度[(46.77±5.02)%],乌司他丁干预组大鼠肺泡Ⅱ型上皮细胞凋亡率及Ca^(2+)浓度显著低于SAP组(P<0.05)。假手术组大鼠Caspasee⁃8、BaxmRNA表达均显著低于SAP组及乌司他丁干预组,乌司他丁干预组大鼠Caspasee⁃8、BaxmRNA表达显著低于SAP组(P<0.05)。SAP肺损伤大鼠线粒体细胞破坏明显,乌司他丁对减少线粒体细胞破坏数量具有明显作用。结论SAP肺损伤中肺泡Ⅱ型上皮细胞凋亡可能参与了其作用机制,TNF⁃α、AMY、MDA、Caspasee⁃8、BaxmRNA在肺损伤机制中存在重要作用,乌司他丁干预有利于缓解SAP肺损伤状况,有利于控制病情进展。

特布他林对肺泡Ⅰ型和Ⅱ型细胞钠水转运机制的影响

目的探讨特布他林对肺泡Ⅰ型细胞(ATⅠ)和Ⅱ型细胞(ATⅡ)上Na+转运机制的影响。方法分离ATⅡ,采用膜片钳全细胞记录模式,应用全细胞钠通道(ENaC)阻断剂amiloride和环核苷酸门控阳离子通道(CNG)阻断剂ZnCl2观察ATⅡENaC和CNG电流及特布他林对两者的影响。结果 ATⅡ全细胞电流主要为amiloride敏感电流和Zn2+敏感电流,两者比例无差别(P>0.05);特布他林可使amiloride敏感电流和Zn2+敏感电流明显增加(P<0.05),amiloride敏感电流所占比例约为Zn2+敏感电流的1.7倍(P<0.05)。结论急性分离ATⅡ上存在功能性ENaC和CNG,并且Na+转运以两者为主。特布他林增强肺水吸收主要通过增加ATⅠ和ATⅡ上ENaC和CNG通道的Na+转运实现。

YY1对肺泡Ⅰ型上皮细胞纤维化的调控研究

目的研究核转录因子YinYang1(YY1)对肺泡Ⅰ型上皮细胞的调控功能及作用机制。方法比较不同肺泡上皮细胞和肺癌细胞中纤维化标志物分子和YY1的表达;通过CCK8增殖实验检测YY1对R3/1细胞增殖的影响;通过YY1过表达以及特异敲低技术,检测TGF-β1刺激R3/1细胞后纤维化标志物分子的表达;通过Western印迹法检测YY1影响NF-κB质核转移的作用。结果纤维化标志物分子α-sma和vimentin在R3/1细胞中特异高表达,与A549细胞相比,YY1在R3/1细胞中低表达; YY1显著抑制R3/1细胞增殖;过表达YY1降低TGF-β1诱导R3/1细胞中的α-sma和vimentin的表达,敲低YY1能够进一步促进TGF-β1诱导的α-sma高表达;在R3/1细胞中过表达YY1抑制TGF-β1诱导的NF-κB细胞核蛋白增加。结论 YY1在R3/1细胞中能够抑制TGF-β1诱导的NF-κB从细胞质到细胞核的转移,进而抑制了其对纤维化基因的转录激活。

转化生长因子β1对体外培养hRPE细胞增殖率及Ⅰ型胶原表达的影响

目的:探讨TGF-β1对体外培养人视网膜色素上皮(human retinal pigment epithelium,hRPE)细胞增殖率及I型胶原表达的影响。方法:实验组用0.1、1、10μg/L的TGF-β1对体外培养hRPE细胞进行干预,对照组只加培养液培养hRPE细胞,用RT-PCR与酶联免疫吸附法检测Ⅰ型胶原mRNA和蛋白表达,用MTT法检测细胞的增殖率。结果:实验组hRPE细胞Ⅰ型胶原的mRNA和蛋白表达量及细胞增殖率较对照组明显增高(P<0.05),1μg/L组进一步升高(P<0.05),10μg/L组达高峰(P<0.05),呈现明显的剂量依赖性,TGF-β1浓度与Ⅰ型胶原蛋白的表达及增殖率的相关系数r分别为0.863及0.901。结论:TGF-β1能够促进hRPE细胞Ⅰ型胶原的表达和细胞的增殖,这种现象与TGF-β1的浓度成正相关。

猪肾上皮细胞Ⅰ型干扰素受体1敲除对伪狂犬病毒复制的影响

目的探讨Ⅰ型干扰素受体1 (IFNAR1)对伪狂犬病病毒(PRV)复制的影响。方法以慢病毒介导的CRISPR/Cas9基因编辑技术,构建猪肾上皮细胞(PK15)敲除IFNAR1基因的稳定细胞系。运用细胞活力检测、荧光观察、流式细胞术检测、滴度测定、Real-time PCR等技术进行IFNAR1功能验证。结果随着PRV感染时间延长,敲除IFNAR1基因可以显著促进PRV-TK mRNA的转录,PRV-gE蛋白的翻译以及子代病毒的毒力。结论IFNAR1在抑制PRV增殖中发挥重要作用。

非编码RNA与特发性肺纤维化进程中的干细胞异常

背景:非编码RNA随着高通量技术的发展而逐渐引发关注,其广泛参与呼吸系统各疾病病程。特发性肺纤维化进程伴随着干细胞功能异常,近来研究表明非编码RNA与干细胞功能异常存在联系,进而影响肺纤维化进展。以非编码RNA为靶点的基因疗法暗示了阻断纤维化过程的可能性。目的:总结非编码RNA在特发性肺纤维化干细胞功能异常和治疗中的研究进展。方法:以“IPF,Stem cells,miRNA,lncRNA,circRNA,treatment”为英文检索词,以“特发性肺纤维化、干细胞、miRNA、lncRNA、circRNA、治疗”为中文检索词,检索PubMed、Wiley InterScience、中国知网和万方数据库,范围囊括近10年的文献,然后依据纳入和排除标准进行筛选,最终纳入82篇文献进行分析。结果与结论:①文章首次总结了近年来非编码RNA在特发性肺纤维化的干细胞异常机制中的相关性研究,揭示了miRNA,lncRNA及circRNA共同调控了干细胞的异常激活、分化等活动,并且miRNA常作为后两者作用的中心环节。②现有的临床试验一定程度上肯定了干细胞移植疗法治疗特发性肺纤维化的安全性,但在疗效方面,仅稍改善了患者弥散功能却未能明确缓解纤维化病变的程度,其结果还需要更多设立安慰剂对照的随机试验来验证。③靶向非编码RNA的基因治疗优势在于具有多基因调控特性,可以从上游干预干细胞异常,目前其在体内外实验已取得突破性进展,并被证实与部分药物的作用靶点相关。④然而,特发性肺纤维化基因疗法的缺点是只能产生短期效应,同时其面临着有效剂量、体内稳定性及输送等问题,这些问题还需未来研究进一步解决。⑤总之,虽然非编码RNA疗法自身存在缺陷,但也不失为一种改善肺纤维化干细胞功能异常的新途径,将其与干细胞移植结合,取长补短,可能发挥更好的疗效。

不同浓度PM_(2.5)对小鼠肺泡Ⅱ型上皮细胞MLE-12的损伤作用及SP-B表达影响

目的探讨不同浓度细颗粒物(PM_(2.5))对小鼠肺泡Ⅱ型上皮细胞MLE-12的损伤作用及肺表面活性蛋白-B(SP-B)表达的影响。方法将肺泡Ⅱ型上皮细胞MLE-12分为实验组和对照组。实验组采用加入12.5、25、50、100、200μg/mL PM_(2.5)混悬液的DMEM完全培养基培养,对照组采用DMEM完全培养基培养。培养24 h或48 h后,采用光学显微镜观察细胞形态,透射电镜观察细胞超微结构,RTCA仪观察细胞增殖能力;Western blotting法检测细胞中SP-B蛋白;qRT-PCR法检测细胞中SP-B mRNA。结果随着PM_(2.5)浓度的升高,实验组细胞形态和超微结构受损程度逐渐加重,可见板层小体受损等细胞器损伤现象,对照组细胞形态和超微结构正常;与对照组相比,PM_(2.5)呈浓度依赖性抑制实验组细胞的增殖。与对照组相比,实验组细胞SP-B蛋白和mRNA表达呈浓度依赖性下调(P均<0.05)。结论PM_(2.5)可呈剂量依赖性损伤小鼠肺泡Ⅱ型上皮细胞MLE-12,并下调SP-B表达。

瘦素/ERK信号在云锡矿粉诱导大鼠II型肺泡上皮细胞转化中的作用

背景与目的目前,云南个旧锡矿有大量矿工从事开采工作,这种职业环境与接触粉尘颗粒、重金属、多环芳烃和放射性氡有关,大大增加了患肺癌的风险。本研究旨在探讨在云锡矿粉诱导大鼠肺泡Ⅱ型上皮细胞(immortalized rat alveolar cells type Ⅱ,RLE-6TN)恶性转化过程中,瘦素(leptin)及其介导的细胞外调节蛋白激酶(extracellular regulated protein kinase,ERK)信号通路所起的作用。方法采用200μg/mL的云锡矿粉隔代毒染RLE-6TN至第9代,建立毒染细胞模型,命名为R_(200)细胞,正常培养组命名为R细胞,通过Western blot法检测两种细胞leptin受体的表达情况。通过MTT法筛选出leptin及丝裂原活化蛋白激酶激酶(mitogen-activated protein kinase kinase,MEK)抑制剂(U0126)对R_(200)细胞的最佳作用浓度。自第20代起,将R组、R_(200)组细胞分别与leptin及MEK抑制剂U0126共培养,对各组细胞的形态改变进行观察,并利用苏木素-伊红(hematoxylin-eosin,HE)染色技术鉴别第40代细胞的形态学差异,通过刀豆凝集素A(concanavalin A,ConA)及锚着独立性生长实验法检测细胞恶性转化情况。通过Western blot法检测leptin作用后上皮细胞ERK信号通路的变化。结果R组和R_(200)组细胞均表达leptin受体(OB-R)。与R_(200)组比较,当leptin浓度达100 ng/mL时,其促增殖效应最为显著,30μmol/L U0126可抑制毒染细胞R_(200)增殖,与对照组相比具有统计学差异(P<0.05)。自第25代起,leptin诱导的R_(200)组(R_(200)L组)细胞形态发生变化,至第30代出现恶性转化,至第40代时恶性转化特征明显;而R_(200)组细胞及U0126诱导的R_(200)组(R_(200)LU组)细胞则在第40代时才出现恶性转化特征。R_(200)L组细胞凝集速度较R_(200)LU组快,其余各组细胞P30出现凝集,且随ConA浓度增加,细胞凝集速度加快。R_(200)L组细胞自P40可见克隆形成,克隆形成率为2.25‰±0.5‰,R_(200)LU组及R_(200)组未见克隆集落。R_(200)L组细胞pERK表达增强;加入U0126阻断后,R_(200)L组细胞pERK磷酸化水平降低。结论Leptin可以促进云锡矿粉毒染肺上皮细胞的恶性转化,ERK信号通路可能是其促进云锡矿粉引发的肺泡Ⅱ型上皮细胞转化的重要途径。