ISOFLURANE REDUCES THE SYNTHESIS OF SURFACTANT-RELATED PROTEIN A OF ALVEOLAR TYPE II CELLS INJURED BY H_2O_2

Objective To explore the influence of isoflurane(Iso) on the synthesis of surfactant-related protein(SP-A) of alveolar type II cells(AT II cells) cultured in primary and injured by hydrogen peroxide(H2O2).Methods AT II cells were isolated from adult SD rats and used for experiments after 32h in primary culture and randomized into six groups: control group,0.28 mM Iso group,2.8mM Iso group,75 μM H2O2 group,75 μM H2O2 +0.28 mM Iso group and 75 μM H2O2 +2.8 mM Iso group. Each group was continuously incubated for 3 h after administration of Iso or/and H2O2. The intracellular SP-A and the SP-A of cultured medium were measured with an enzyme-linked immunosorbent assay(ELISA).Results Iso significantly decreased SP-A content of cultured medium and the intracellular,and aggravated the decrease of SP-A content induced by H2O2 in a dose-dependent manner.Conclusion Iso itself may decrease SP-A synthesis of AT II cells in vitro,and aggravate the damage of AT II cells especially under peroxidation condition.

Diagnostic value of gamma-glutamyltransferase/aspartate aminotransferase ratio, protein induced by vitamin K absence or antagonist II, and alpha-fetoprotein in hepatitis B virus-related hepatocellular carcinoma

BACKGROUND Researchers have investigated the diagnostic value of protein induced by vitamin K absence or antagonist II (PIVKA-II) and alpha-fetoprotein (AFP) in hepatitis B virus (HBV)-related hepatocellular carcinoma (HCC), and obtained abundant clinical diagnostic data. However, PIVKA-II and AFP have unsatisfactory specificity and sensitivity in the diagnosis of early-stage HBV-related HCC. Gamma-glutamyltransferase (γ-GT) and aspartate aminotransferase (AST) are common biomarkers for evaluating liver function, and we hypothesized that the γ-GT/AST ratio in combination with PIVKA-II and AFP would improve the diagnosis of early-stage HBV-related HCC. AIM To evaluate the diagnostic value of γ-GT/AST ratio alone or in combination with PIVKA-II and AFP in HBV-related HCC. METHODS Serum levels of γ-GT, AST, PIVKA-II, and AFP were detected and analysed in 176 patients with HBV-related HCC and in 359 patients with chronic hepatitis B. According to tumour size and serum level of HBV DNA, HBV-related HCC patients were divided into the following categories: Early-stage HCC patients, HCC patients, HBV DNA positive (HBV DNA+) HCC patients, and HBV DNA negative (HBV DNA-) HCC patients. Receiver-operating characteristic (ROC) curves were used to analyse and compare the diagnostic value of the single and combined detection of various biomarkers in different types of HBV-related HCC. RESULTS Tumour size was positively correlated with serum levels of PIVKA-II and AFP in HCC patients (r = 0.529, aP < 0.001 and r = 0.270, bP < 0.001, respectively), but there was no correlation between tumour size and the γ-GT/AST ratio (r = 0.073, P = 0.336). The areas under the receiver-operating characteristic curves (AUROCs) of the γ-GT/AST ratio in early-stage HCC patients, HBV DNA+ HCC patients and HBV DNA- HCC patients were not significantly different from that in the total HCC patients (0.754, 0.802, and 0.705 vs 0.779, respectively;P > 0.05). When PIVKA-II was combined with the γ-GT/AST ratio in the diagnosis of earlystage HCC, HCC, and HBV DNA+ HCC, the AUROCs of PIVKA-II increased, with values of 0.857 vs 0.835, 0.925 vs 0.913, and 0.958 vs 0.954, respectively. When AFP was combined with the γ-GT/AST ratio in the diagnosis of early-stage HCC, HCC, HBV DNA+ HCC, and HBV DNA- HCC, the AUROCs of AFP increased, with values of 0.757 vs 0.621, 0.837 vs 0.744, 0.868 vs 0.757, and 0.840 vs 0.828, respectively. CONCLUSION The γ-GT/AST ratio may be better than PIVKA-II and AFP in the diagnosis of early-stage HBV-related HCC, and its combination with PIVKA-II and AFP can improve the diagnostic value for HBV-related HCC.

Ca2+/calmodulin-dependent protein kinase II regulates colon cancer proliferation and migration via ERK1/2 and p38 pathways

AIM To investigate the role of calmodulin-dependent protein kinase Ⅱ(Ca MKⅡ) in colon cancer growth,migration and invasion.METHODS Ca MKⅡ expression in colon cancer and paracancerous tissues was evaluated via immunochemistry. Transcriptional and posttranscriptional levels of Ca MKⅡin tissue samples and MMP2,MMP9 and TIMP-1 expression in the human colon cancer cell line HCT116 were assessed by q RTPCR and western blot. Cell proliferation was detected with the MTT assay. Cancer cell migration and invasion were investigated with the Transwell culture system and woundhealing assay.RESULTS We first demonstrated that CaMK Ⅱ was ove rexpressed in human colon cancers and was associated with cancer differentiation. In the human colon cancer cell line HCT116,the Ca MKII-specific inhibitor KN93,but not its inactive analogue KN92,decreased cancer cell proliferation. Furthermore,KN93 also significantly prohibited HCT116 cell migration and invasion. The specific inhibition of ERK1/2 or p38 decreased the proliferation and migration of colon cancer cells.CONCLUSION Our findings highlight Ca MKⅡ as a potential critical mediator in human colon tumor development and metastasis.

The calmodulin-dependent protein kinase II inhibitor KN-93 protects rat cerebral cortical neurons from N-methyl-D-aspartic acid-induced injury

In this study, primary cultured cerebral cortical neurons of Sprague-Dawley neonatal rats were treated with 0.25, 0.5, and 1.0 μM calmodulin-dependent protein kinase II inhibitor KN-93 after 50 μM N-methyI-D-aspartic acid-induced injury. Results showed that, compared with N-methyi-D- aspartic acid-induced injury neurons, the activity of cells markedly increased, apoptosis was significantly reduced, leakage of lactate dehydrogenase decreased, and intracellular Ca2＋ concentrations in neurons reduced after KN-93 treatment. The expression of caspase-3, phosphorylated calmodulin-dependent protein kinase II and total calmodulin-dependent protein kinase II protein decreased after KN-93 treatment. And the effect was apparent at a dose of 1.0 pM KN-93. Experimental findings suggest that KN-93 can induce a dose-dependent neuroprotective effect, and that the underlying mechanism may be related to the down-regulation of caspase-3 and calmodulin- dependent protein kinase II expression.

Effect of gestational protein restriction on left ventricle hypertrophy and heart angiotensin II signaling pathway in adult offspring rats

Maternal protein restriction may be a risk factor for cardiovascular disorders in adulthood. The RAS (renin-angiotensin-system) plays a pivotal role in cardiac remodeling. Components of the RAS, including angiotensin II (AngII) and its receptors type 1 (AT1R) and 2 (AT2R) are expressed in the heart. This study investigates whether gestational protein restriction alters the expression and localization of AT1R and AT2R and RAS signaling pathway proteins in parallel with left ventricle hypertrophy and systemic hypertension in male offspring. Dams were kept on normal (NP, 17% protein) or low (LP, 6% protein) protein diet during pregnancy. Systolic blood pressure (SBP) of male offspring was measured from the 8th to 16th week and left ventricles of 16-wk-old rats were processed for histology, morphometric, immunoblotting and immunohistochemistry. LP offspring showed a significant reduction in birth body weight and SBP increased significantly from the 8th week. Left ventricle mass and cardiomyocytes area were also significantly higher in LP animals. Widespread perivascular fibrosis was not detected in the heart tissue. Analysis by immunoblotting and immunohistochemistry demonstrated a significant enhance in cardiomyocyte expression of AT1R and ERK1 in LP offspring. Expression of PI3K in LP was significantly reduced in cardiomyocytes and in the intramural coronary wall, while AT2R expression was unchanged in the NP group. We also found reduced LP expression of JAK2 and STAT3. In conclusion, our data also suggest that changes in the RAS may play a role in the ventricular growth through upregulation of the AT1-mediated ERK1/2 response, despite unchanged AT2R expression.

A SENSITIVE PROTEIN ASSAY BY Co(II)-BIURET METHOD

A new and senseitive Co (II)-biuret method for determination of protein has for the first time been established. In visible wavelength region, the Co (II) -protein complexes had anabsorption peak at 360 nm. -Under the present conditions. the assay had a linear range of 0-120 μg/ml of protein with a detection limit of about 2 μg/ml, and similar calibration curves were obtained for BSA. and BγG. Compared with Cu (II) -biuret method, the present Co (II) -biuret method was more simple, sensitive, and tolerant of interferences from non-protein molecules.

阴道镜直视下宫颈活检诊断CINII中漏诊CINII以上病变的研究及意义

目的:评价阴道镜直视下活检诊断CINII的准确性,分析影响漏诊CINII以上病变(简称CINII^+)的相关因素,并探讨P16^(INK4a)蛋白表达在预测漏诊CINII^+中的价值。方法:回顾分析2013年12月至2015年7月在南京医科大学第一附属医院宫颈病中心阴道镜直视下宫颈活检诊断为CINII,且在短期内行LEEP的148例患者。研究患者手术前后病理诊断,同时对患者年龄、初次TCT结果、高危型HPV负荷量、阴道镜下病变累及宫颈象限数、转化区类型、阴道镜图像表现以及CINII组织中P16^(INK4a)蛋白表达等与漏诊CINII^+的关系进行单因素及多因素分析。结果:(1)阴道镜直视下活检诊断的148例CINII中,71例(49.97%)漏诊CINII^+,其中1例宫颈鳞癌IA1期,1例宫颈鳞癌IB1期。单因素分析显示,患者年龄、初次TCT结果、高危型HPV负荷量、阴道镜下病变累及象限数、转化区类型、阴道镜图像特征与CINII^+病变漏诊无明显相关性(P>0.05),CINII组织中P16^(INK4a)蛋白表达与CINII^+病变漏诊明显相关(P<0.05)。多因素分析显示,P16^(INK4a)蛋白阳性表达是影响阴道镜直视下活检诊断CINII漏诊CINII^+的危险因素(OR=9.846,95%CI为2.165~44.787;P=0.003)。(2)21例(14.19%)P16^(INK4a)蛋白呈阴性表达,127例(85.81%)呈阳性表达。P16^(INK4a)蛋白表达阴性组中漏诊CINII^+3例(14.29%),P16^(INK4a)蛋白表达阳性组中漏诊CINII^+68例(53.54%),两组比较差异有统计学意义(P<0.05)。P16^(INK4a)阳性表达预测漏诊CINII^+的敏感性95.77%,特异性为23.38%,阴性预测值为85.71%,阳性预测值为53.54%。结论:阴道镜直视下活检诊断的CINII中存在CINII^+的漏诊,而CINII并P16^(INK4a)蛋白阳性表达是影响CINII^+漏诊的危险因素,对P16^(INK4a)蛋白表达阳性的CINII患者的临床干预存在其合理性。针对CINII的个体化管理,需综合考虑患者的年龄、P16^(INK4a)蛋白表达、对生育功能保护的需求及随访的依从性。

恶性疟原虫组氨酸富集蛋白II基因克隆及测序

目的:比较恶性疟原虫不同分离株组氨酸富集蛋白II( HRPII)基因全编码区核苷酸序列。方法: PCR扩增恶性疟原虫海南株(FCC1/HN)和越南株(VN)的HRPII基因全编码区, 其产物经HindIII和Bam HI双酶切,定向克隆入pUC19, 采用Sanger 双脱氧链末端终止法测序。结果:FCC1/HN 株和VN 株HRPII基因均为1 020bp, 无内含子, 两者仅10 个碱基不同。FCC1/HN 株HRPII与VN 株、IMTM22 株和Itg2 株间氨基酸同源性分别为98.8% 、92.2% 和98.7% ; 4 株虫体均有拷贝数不等的丙氨酸-组氨酸-组氨酸(AHH)和丙氨酸-组氨酸-组氨酸-丙氨酸-丙氨酸-天冬氨酸(AHHAAD) 重复序列, 具有相同的信号肽和糖基化位点。4 个分离株HRPII抗原表位相同,位于易曲性较高的5端非AHH 和AHHAAD 重复区。结论: FCC1/HN 株与VN 株的HRPII高度同源,与IMTM22 株和Itg2

植物光系统II放氧复合体外周蛋白结构和功能的研究进展

光合放氧是植物光系统II(PSII)的重要功能之一。PSII的放氧反应主要是由PSII氧化侧的 4个锰原子组成的锰簇催化的。在类囊体膜的囊腔侧还结合有若干个外周蛋白 ,对放氧反应起着重要作用。

光系统II蛋白磷酸化及其生理意义

蛋白磷酸化修饰在几乎所有的生命活动中都起重要的调节作用。该文结合作者研究组的研究工作 ,概述了光系统II(PSII)蛋白磷酸化的调节及其生理功能。PSII复合体中的核心组分D1、D2、CP43和PsbH蛋白以及外周捕光天线 (LHCII)蛋白都可以发生磷酸化。PSII蛋白磷酸化受质醌 (PQ)的氧化还原状态、细胞色素b6f(Cytb6f)和硫氧还蛋白以及光调节。PSII蛋白磷酸化可以调节激发能在两种光系统(PSI和PSII)之间的分配 ,减轻光胁迫对PSII的压力 ,保护核心蛋白免于光破坏 ,稳定PSII复合体的结构。

rhBMP-2在体内诱导成骨中I,II型胶原及碱性磷酸酶的表达

目的 对 rh BMP- 2在诱导成骨中 Collagen I,II及碱性磷酸酶 (AL P)的表达进行研究 .方法 将含 rh BMP- 2 0 .5mg的松质骨载体植入 5 5只 BAL B/ c小鼠的右侧股部肌袋内 ,分别于术后 3～ 2 1d共 8个时间点取材 ,采用免疫组织化学方法对新生骨组织中的 I,II型胶原进行检测 ;对 AL P活性进行定量分析 ,观察 rh BMP- 2在诱导成骨中 Collagen I,II及AL P的表达情况 .结果 1II型胶原的出现是和成软骨、软骨细胞的出现相伴随的 ,但是 ,肥大、变性的软骨细胞并不表达 II型胶原 ;2作为成骨细胞成熟标志物的 I型胶原、AL P在软骨形成期即有表达 ,但是随着成骨细胞的出现 ,骨组织的形成 I型胶原仍表现为高表达 ,而 AL P的表达则呈下降趋势 .结论 在诱导成骨中 rh BMP- 2促进了 Collagen I,II及AL P的表达 .

阿片类药物对NG108-15细胞Ca^(2+)/钙调蛋白依赖的蛋白激酶II信息通路的作用

目的 观察阿片类依赖时Ca2 + 钙调蛋白依赖的蛋白激酶II信息通路的变化。方法 以NG10 8 15细胞作为体外的细胞模型 ,分别用竞争性蛋白结合法及放射免疫法、PDE法、γ 32 P参入法测定cAMP水平、钙调蛋白(CaM)活性和钙调蛋白依赖的蛋白激酶II(CaMKII)活性。结果 DPDPE作用NG10 8 15细胞 48h可使细胞浆和细胞核CaM和CaMKII活性升高 ,该变化可被CaM特异性拮抗剂W 7所抑制 ;CaMKII特异性抑制剂KN 6 2可抑制CaMKII活性的增高 ,而对CaM活性无明显影响。DPDPE作用NG10 8 15细胞 48h后 ,加入纳洛酮 ,CaM活性、CaMKII活性进一步增高。结论 Ca2 + CaMKII信息通路参与了阿片依赖的机制。

芜菁花叶病毒外壳蛋白在寄主植物叶绿体中的积累及其对光系统II活性的影响

分别以接种感染芜菁花叶病毒(TuMV)和健康对照的青菜苏州青品种(Brassica chinensis L. cv.Suzhou)和芥菜温州芥菜品种(B.juncea L. cv.Wenzhou)叶片为材料提取完整叶绿体,用胰蛋白酶消除其表面蛋白后,抽提总蛋白,经SDS-PAGE电泳和Western blot检测,发现TuMV的外壳蛋白(CP)存在于感病寄主的叶绿体中。免疫金标记电镜实验显示TuMV-CP定位在感病青菜和芥菜的细胞质和叶绿体中。对两种寄主植物叶片的叶绿素荧光动力学参数测定结果显示,青菜、芥菜的Fv/Fo、Fv/Fm、φPSII、qp值都有不同程度的降低,qN值增大。实验结果表明TuMV侵染后在寄主细胞叶绿体中积累的CP,抑制了光系统II(PS II)的光化学活性,这可能是影响寄主植物光合作用的一个重要原因。

p21和IGF-II在肝癌、肝硬化组织中表达的研究

目的 探讨 p2 1、IGF II在肝硬化、肝细胞癌 (HCC)中表达的意义及其与肝细胞不典型增生(LCD)的关系。方法 用免疫组化S P法检测单纯肝硬化、癌旁肝硬化及肝细胞癌 (HCC) p2 1、IGF II表达情况。结果 p2 1、IGF II在癌旁肝硬化和单纯肝硬化组织中的阳性表达率 (92 .86 %和 75 % ;6 8%和 74 % )与HCC(5 4 .5 5 %和 36 .36 % )相比差别有显著性意义 (P <0 .0 5 )。IGF II与p2 1阳性表达存在相关关系。HBsAg阳性或伴LCD改变的肝硬化 ,p2 1、IGF II阳性率均高于HBsAg阴性或不伴有LCD改变的肝硬化 (P <0 .0 5 )。结论 (1)在肝细胞癌变演化过程中 p2 1、IGF II可能发挥协同作用。 (2 )LCD可能是一群具有肿瘤增殖潜能的癌前细胞群 ,尤其有 p2 1、IGF II共同过度表达者 ,有发生HCC的高度危险。

小鼠spindlin1蛋白在稳定MII期卵母细胞纺锤体中的作用

目的目的探讨小鼠spindlin1蛋白在MII期卵母细胞中的作用。方法采用免疫荧光方法对spindlin1蛋白在小鼠卵母细胞中的定位进行研究。采用抗体显微注射实验对其在MII期卵母细胞中的功能进行了研究。结果免疫荧光结果显示在MII期,spindlin1蛋白定位于中期纺锤体,当卵母细胞进入分裂后期,spindlin1蛋白从纺锤体上消失。抗体注射实验显示在MII期卵母细胞中干扰spindlin1蛋白后,纺锤体形态明显异常且染色体排列发生紊乱。结论小鼠spin-dlin1蛋白在MII期卵母细胞中发挥作用,参与维持中期纺锤体的稳定,保障了染色体的正确分离。

CKII抑制剂——肝癌治疗新靶点

目的探讨蛋白激酶(casein kinase 2,CK2)抑制剂影响肝癌细胞株HepG-2凋亡的机制,为其临床治疗肝癌提供可能的实验依据。方法本研究通过MTT法和流式细胞仪检测和观察不同作用时间、不同浓度CK2抑制剂四溴苯三唑(4,5,6,7-tetrabromobenzotriazole,TBB)作用HepG-2肝癌细胞株后对其增殖和凋亡的影响,分别应用荧光定量PCR和Western blot实验分析可能机制。结果 TBB在48 h浓度为200μmol/L时对肝癌细胞的抑制作用最明显;150μmol/L TBB作用48 h后,早期凋亡率明显增高,至(13.2±0.67)%,磷酸化P65在100μmol/L TBB实验组表达下调,而caspase-3、caspase-8、Bcl-2和Bcl-x等在两组间表达未见明显差异。结论 CK2抑制剂TBB能够通过参与调控NF-κB信号转导通路抑制肿瘤细胞增殖,促进其凋亡,可能成为未来肝癌治疗的一个新的靶点。

血管紧张素II对心肌细胞蛋白质合成速率和肌球蛋白重链基因表达的作用

目的：研究血管紧张素ＩＩ（ＡｎｇＩＩ）对心肌细胞蛋白质合成速率和肌球蛋白重链（ｍｙｏｓｉｎｈｅａｖｙｃｈａｉｎ，ＭＨＣ）基因表达的影响。方法：采用放射性同位素氚（３Ｈ）－亮氨酸参入量方法观察培养心肌细胞蛋白质合成速率。应用斑点杂交方法分析ＡｎｇＩ对心肌细胞α－ＭＨＣ和β－ＭＨＣ基因表达的作用。结果：在培养的心肌细胞中加入ＡｎｇＩ可明显增加心肌细胞３Ｈ－亮氨酸的参入量，并可诱导心肌细胞α－ＭＨＣ和β－ＭＨＣ基因表达迅速增加，在一定范围内，两者均呈量效关系。ＡｎｇＩ阻断剂沙拉新（ｓａｒ－ａｌａｓｉｎ）可阻断ＡｎｇＩＩ的上述作用。结论：ＡｎｇＩＩ可增加心肌细胞蛋白质合成速率，促进心肌细胞α－ＭＨＣ和β－ＭＨＣ基因表达。

抗环子孢子蛋白保守II^+区单克隆抗体的制备及鉴定

目的 获得针对恶性疟原虫环子孢子蛋白 (CSP)保守II+ 区 (RegionII+ )的单克隆抗体。 方法 采用恶性疟原虫保守II+ 区十二肽 (EWSPCSVTCGNG)免疫BALB/c小鼠 ,经融合 ,ELISA 3次筛选 ,获得 3株分泌针对保守II+ 区单克隆抗体的杂交瘤细胞株。 结果 ELISA检测结果显示单抗能与重组表达的恶性疟原虫CSP片段及天然CSP特异性反应。间接荧光抗体检测显示 ,单抗不仅能识别恶性疟原虫子孢子 ,也能识别约氏疟原虫子孢子。 结论 成功地获得了针对恶性疟原虫CSP保守II+

太子健II缓解期防治小儿哮喘作用机理的实验研究

运用鸡卵蛋白致敏和反复诱喘的哮喘豚鼠模型,将豚鼠随机分为正常组、模型组、地塞米松组、高剂量和低剂量组5组,观察太子健II对其血及气道内嗜酸细胞浸润和血中白介素-5(IL-5)、嗜酸粒细胞阳离子蛋白(ECP)含量的影响.结果表明太子健II可减少哮喘豚鼠血及气道内EOS浸润,降低血中白介素-5(IL-5)和ECP的水平.说明太子健II可以减轻气道慢性变应性炎症,具有一定的抗哮喘复发的作用.

PTSD大鼠杏仁核CaMKIIα及pCaMKIIα表达的变化

目的观察创伤后应激障碍(PTSD)样行为异常大鼠杏仁核神经元CaM依赖性蛋白激酶IIα(CaMKIIα)及磷酸化CaM依赖性蛋白激酶IIα(pCaMKIIα)表达变化。方法采用国际认定的SPS方法刺激建立大鼠PTSD模型,取成年健康雄性Wistar大鼠75只,随机分为SPS模型的12h、1d、4d、7d组及正常对照组,采用免疫组织化学、免疫印迹法检测大鼠杏仁核CaMKIIα及pCaMKIIα的表达变化。结果SPS刺激后大鼠杏仁核神经元细胞内CaMKIIα于12h开始减少,1d表达最少,4d开始逐渐增多,至7d时基本恢复正常;pCaMKIIα的表达则于SPS12h开始增多,1d时表达最多,4d时开始减少,至7d时基本恢复正常。CaMKIIα阳性细胞在SPS各组模型均出现,1d表达最少。结论杏仁核CaMKIIα及pCaMKIIα的表达变化,可能是PTSD大鼠情感行为异常的重要病理生理基础之一。