CircACAP2靶向miR-29a-3p/CCNT2轴对缺氧/复氧诱导的心肌细胞损伤的影响

目的:探讨CircACAP2靶向miR-29a-3p/细胞周期蛋白T2(CCNT2)轴对缺氧/复氧(H/R)诱导的心肌细胞损伤的影响。方法:将H9c2细胞分为Control组(正常培养)、si-NC组(转染si-NC)、Model组(建立H/R模型)、si-CircACAP2组(转染si-CircACAP2)、si-CircACAP2+inhibitor-NC组(si-CircACAP2和inhibitor-NC共转染)、si-CircACAP2+miR-29a-3p inhibitor组(si-CircACAP2和miR-29a-3p inhibitor共转染);实时荧光定量聚合酶链式反应(qRT-PCR)检测H9c2细胞中CircACAP2、miR-29a-3p的表达水平;四唑盐(MTT)法检测H9c2细胞活力;流式细胞仪检测H9c2细胞凋亡;单丹磺酰尸胺(MDC)染色法检测H9c2细胞自噬;乳酸脱氢酶(LDH)、丙二醛(MDA)、超氧化物歧化酶(SOD)试剂盒检测H9c2细胞上清中LDH、MDA、SOD水平,DCFH-DA荧光探针法检测细胞内活性氧(ROS)水平;蛋白质免疫印迹法(Western Blot)检测增殖细胞核抗原(PCNA)、细胞凋亡蛋白[B细胞淋巴瘤/白血病-2(Bcl-2)、Bcl-2相关X蛋白(Bax)]、自噬相关蛋白(Beclin-1、P62)及CCNT2的表达;双荧光素酶报告检测CircACAP2对miR-29a-3p的靶向关系和miR-29a-3p对CCNT2的靶向关系。结果:与Control组比较,Model组H9c2细胞中CircACAP2表达、凋亡率、自噬囊泡数、LDH释放率、MDA、ROS水平、Bax、Beclin-1、CCNT2蛋白表达升高,miR-29a-3p表达、OD490值、SOD活性、PCNA、Bcl-2、P62蛋白表达降低(P<0.05);与Model组比较,si-CircACAP2组H9c2细胞中CircACAP2表达、凋亡率、自噬囊泡数、LDH释放率、MDA、ROS水平、Bax、Beclin-1、CCNT2蛋白表达降低,miR-29a-3p表达、OD490值、SOD活性、PCNA、Bcl-2、P62蛋白表达升高(P<0.05);与si-CircACAP2组比较,si-CircACAP2+miR-29a-3p inhibitor组H9c2细胞中CircACAP2表达差异无统计学意义(P>0.05),凋亡率、自噬囊泡数、LDH释放率、MDA、ROS水平、Bax、Beclin-1、CCNT2蛋白表达升高,miR-29a-3p表达、OD490值、SOD活性、PCNA、Bcl-2、P62蛋白表达降低(P<0.05);CircACAP2靶向调控miR-29a-3p的表达,miR-29a-3p靶向负调控CCNT2的表达。结论:敲低CircACAP2可能通过靶向miR-29a-3p来下调CCNT2表达,进而抑制H/R诱导的H9c2细胞凋亡、自噬能力及氧化应激,促进细胞增殖,发挥保护作用。

聚氨酯泡沫固定产脂肪酶粗状假丝酵母(Candida valida T2)细胞的研究

对聚氨酯泡沫固定产脂肪酶粗状假丝酵母(Candida valida T2)细胞的固定化条件进行了研究。实验结果表明,聚氨酯泡沫颗粒经密度和粒径筛选,酸碱处理,以及固液比优化,载体固定细胞干质量比达到1 571 mg/g,细胞脂肪酶的酶活为每克干细胞1 415 U。电镜图片显示粗状假丝酵母菌(Candida validaT2)在载体孔隙内和脊壁上缠绕充盈,生长良好,固定结构稳定。固定化细胞连续催化水解桐籽油5批次,细胞相对水解酶活保持率达73%,固定细胞的损失率为12.5%。固定化细胞颗粒显示出良好的操作稳定性和酶活保持率,为进一步的应用研究提供了实验基础。

T2毒素对小鼠外周血象和骨髓造血干、祖细胞的作用

T2毒素2.3 mg/kg(相当LD_(30))单次ip后测定小鼠外周血象,BMNC及骨髓CFUs、CFU—GM、CFU—E和BFU—E的改变以了解T2毒素血液毒理的特征.外周血中WBC总数明显减少,RBC和pt无变化.T2毒素虽不影响CFUs的数量,但对CFU—GM、CFU—E和BFU—E均有杀伤作用,中毒后2 h三种细胞存活率达最低值分别为正常的27％、48％和57％,恢复速度甚快,5 d内全部正常.三种细胞的T2毒素剂量活存曲线均为指数坪型.分析了各类造血干细胞对T2毒素敏感性不同的原因可能与各种细胞固有特性和细胞增殖状态有关。

circ_0001946靶向miR-1270/Cyclin T2轴调控胃癌细胞恶性表型的分子机制研究

目的探讨circ_0001946对胃癌细胞恶性表型的影响及可能机制。方法采用qRT-PCR法检测胃癌组织和细胞系(HGC-27、AGS、MKN45)中circ_0001946和miR-1270表达情况,并采用Pearson相关性分析探讨胃癌组织中circ_0001946和miR-1270表达的相关性。分别转染circ_0001946小干扰RNA、miR-1270模拟物或共转染circ_0001946小干扰RNA与miR-1270抑制剂至胃癌HGC-27细胞,采用CCK-8法和克隆形成实验检测细胞增殖情况,采用流式细胞术检测细胞凋亡情况,采用Transwell法检测细胞侵袭情况,采用蛋白免疫印迹法检测细胞周期蛋白T2(Cyclin T2)表达情况。行双荧光素酶报告基因实验验证circ_0001946、miR-1270和Cyclin T2调控的关系。结果胃癌组织和细胞系中circ_0001946表达升高(P<0.05),而miR-1270表达降低(P<0.05),且胃癌组织中circ_0001946与miR-1270表达呈负相关(r=-0.752,P<0.05)。敲减circ_0001946过表达后HGC-27细胞光密度(OD)值、克隆形成数和侵袭数降低(P<0.05),而凋亡率升高(P<0.05)。敲减miR-1270过表达后可升高HGC-27细胞OD值、克隆形成数和侵袭数(P<0.05),降低凋亡率(P<0.05)。circ_0001946可竞争性结合miR-1270,Cyclin T2是miR-1270的靶基因。结论circ_0001946在胃癌组织和细胞系中表达升高,其可能通过靶向miR-1270/Cyclin T2轴促进胃癌细胞增殖和侵袭,并诱导胃癌细胞凋亡,有可能成为胃癌治疗的分子靶点。

非阻断肾动脉腹腔镜肾部分切除术治疗T1～T2期肾癌

目的探讨非阻断肾动脉腹腔镜肾部分切除术治疗T1~T2期肾癌的效果与安全性。方法回顾性分析2012年1月至2016年5月在我院诊治的140例T1~T2期肾癌患者的临床资料,根据治疗方法的不同分为观察组与对照组,每组70例。观察组实施腹腔镜下非阻断肾动脉肾部分切除术,对照组实施腹腔镜下选择性阻断肾动脉肾部分切除术,记录2组患者围手术期情况、术后并发症、术后恢复情况与肾功能变化情况。结果所有患者均完成手术,无中转开腹情况;观察组的手术时间、术中出血量、胃肠恢复时间与术后住院时间明显少于对照组(P<0.05),2组患者的术后引流量与引流管留置时间比较差异无统计学意义(P>0.05)。观察组术后1周的继发性出血、尿漏、肺部感染、切口感染、肾周感染等并发症发生率为2.9%,对照组为15.7%,观察组明显少于对照组(P<0.05)。观察组与对照组术后1周的血清SCr值分别为(89.24±11.92)μmol/L和(117.24±11.49)μmol/L,都明显高于术前的(67.24±12.49)μmol/L和(68.14±13.11)μmol/L(P<0.05),观察组术后1周的血清SCr值也明显少于对照组(P<0.05)。所有患者随访至今,观察组与对照组的中位生存时间分别为(25.32±3.14)个月和(19.39±4.10)个月,观察组明显长于对照组(t=4.209,P<0.05)。结论非阻断肾动脉腹腔镜肾部分切除术治疗T1~T2期肾癌可以避免热缺血,减少术后并发症的发生,保护肾功能,延长患者生存时间。

人多肽:N-乙酰氨基半乳糖转移酶2(ppGalNAc-T2)RNA干扰载体的构建及鉴定

目的:构建稳定的转染人多肽:N-乙酰氨基半乳糖转移酶2(ppGalNAc-T2)基因的RNA i载体。方法:遵循RNA干扰目标序列的选取原则,对ppGalNAc-T2基因mRNA序列设计五条可能的小干扰RNA(siRNA),PCR方法扩增得到siRNA内源表达系统,转染至人胃癌细胞株SGC7901,运用RT-PCR方法检测筛选得到其中能高效引起ppGal-NAc-T2基因表达沉默的siRNA;化学合成带荧光标记的该段RNA O ligo,转染细胞并用荧光显微镜观察转染情况,进一步鉴定该siRNA对ppGalNAc-T2的抑制作用;构建ppGalNAc-T2的RNA干扰真核表达载体,酶切及测序鉴定后转染SGC7901细胞并经G418筛选得到稳定的ppGalNAc-T2基因敲减细胞株,RT-PCR方法检测该转染细胞株ppGalNAc-T2表达水平。结果:采用RNA i技术,将高表达ppGalNAc-T2的SGC7901细胞的T2表达水平明显降低。结论:成功构建稳定的ppGalNAc-T2基因敲减细胞株,为今后进一步深入研究ppGalNAc-T2的生物学功能奠定了基础。

磁共振T2WI信号强度联合DWI-ADC值在肾透明细胞癌与乏脂型肾血管平滑肌脂肪瘤鉴别诊断中的应用

目的分析磁共振成像(MRI)T2加权图像(T2WI)信号强度(SI-T2)比值联合扩散加权成像(DWI)-表观扩散系数(ADC)比值在肾透明细胞癌(ccRCC)与乏脂型肾血管平滑肌脂肪瘤(fpAML)鉴别诊断中的应用意义。方法回顾性分析2021年3月至2024年3月我院收治的接受术前常规MRI检查并经手术标本病理学证实的ccRCC患者62例(设为ccRCC组)和fpAML患者45例(设为fpAML组)的临床资料。全部患者均于术前行MRI平扫和DWI序列扫描,记录MRI征象,同时测量并计算SI-T2比值(肿瘤SI-T2/同侧正常肾皮质SI-T2)和DWI-ADC比值(肿瘤DWI-ADC值/同侧正常肾皮质DWI-ADC值)。采用受试者工作特性曲线(ROC)评价MRI SI-T2比值、DWI-ADC比值单独及联合鉴别诊断ccRCC与fpAML的效能。结果62例ccRCC患者病灶最大径为1.20~6.20(2.90±0.58)cm;36例(58.06%)病灶最大径<4.00cm,均属实性肿块,26例(41.94%)病灶最大径≥4.00cm,主要表现为以实性为主的囊实性肿块,ccRCC实性部分T1WI呈等低信号,T2WI呈略高或混杂等高信号,DWI呈稍高信号。45例fpAML患者病灶最大径0.85~4.30(1.80±0.36)cm;病灶均为实性肿块,信号略欠均匀,T1WI呈等低信号,T2WI以等或略低信号为主,DWI呈稍高信号。ccRCC组病灶最大径显著高于fpAML组(P<0.001)。ccRCC组MRI SI-T2比值显著高于fpAML组(P<0.001),DWI-ADC比值显著低于fpAML组(P<0.05)。ROC曲线分析显示,MRI SI-T2比值、DWI-ADC比值对ccRCC与fpAML均有一定鉴别诊断效能,曲线下面积分别为0.747、0.809;两项联合鉴别诊断ccRCC与fpAML的曲线下面积为0.890。结论MRI SI-T2比值、DWI-ADC比值均能有效鉴别诊断ccRCC与fpAML,而两项联合可进一步提高鉴别诊断效能,值得临床验证。

后腹腔镜肾癌根治术对于T2期肾癌的临床治疗价值探讨

目的：探讨后腹腔镜肾癌根治术对于T2期肾癌的临床治疗价值。方法选取2010年1月～2011年1月期间在我院接受治疗的60例T2期肾癌患者，随机分为实验组与对照组。实验组以后腹腔镜肾癌根治术进行治疗；对照组以开放式肾癌根治术进行治疗。判定后腹腔镜肾癌根治术对于T2期肾癌的临床治疗价值。结果60例患者手术均得以顺利实施，其中，实验组患者的手术平均时长约为（130.2±20.5）min；术中平均失血量为（130.5±10.0）mL；术后平均住院时长为（6.5±3.5）d。术后1年随访，仅1例患者发生疾病复发情况，其他患者均恢复良好；对照组患者手术平均时长为（165.8±30.2）min；术中平均失血量为（175.5±12.2）ml；术后平均住院时长为（15.5±4.2）d。术后1年随访，6例患者发生疾病复发情况。两组数据差异显著，结果具有统计意义（P＜0.05）。结论后腹腔镜肾癌根治术具有较高的临床治疗价值，其手术耗时短、患者术中出血量少、术后住院时间短、复发率低，该手术法值得在临床上广泛推广，帮助更多的肾癌患者受益。

后腹腔镜肾癌根治术对T2期肾癌患者的临床疗效和安全性分析

目的观察后腹腔镜肾癌根治术对T2期肾癌的临床疗效和安全性。方法方便选取2015年1月—2018年1月收治的T2期肾癌患者92例分为两组:试验组予以后腹腔镜肾癌根治术;对照组予以开放式肾癌根治术。比较两组的手术相关指标、疗效和炎性因子。结果试验组术中出血量、术后拔管时间、住院时长、术后Hs-CRP、TNF-α、IL-6低于对照组[(110.92±28.18)mLvs(231.29±41.21)mL(t=16.452,P=0.003);(2.23±1.08)dvs(4.04±1.42)d(t=5.976,P=0.006);(7.28±2.12)dvs(9.90±2.57)d(t=4.139,P=0.009);(16.63±3.22)mg/Lvs(23.35±4.56)mg/L(t=4.054,P=0.011);(46.71±13.73)mg/mLvs(58.56±18.29)mg/mL(t=4.338,P=0.013);(26.27±6.18)pg/mLvs(35.98±10.11)pg/mL(t=3.658,P=0.036),差异有统计学意义(P<0.05)。结论后腹腔镜肾癌根治术与开放式肾癌根治术的临床疗效一致,对患者造成的创伤小、机体炎症反应低、患者恢复快,安全性佳。

首发精神分裂症患者前额叶皮质背外侧-腹内侧T2信号强度与外周血白细胞的研究

目的:探讨首发精神分裂症患者前额叶皮质背外侧(DLPFC)-腹内侧(VMPFC)的T2信号强度与外周血白细胞(WBC)水平的关系。方法:35例首发精神分裂症患者(患者组)与35名健康志愿者(对照组)均接受3.0 T磁共振(MRI)头部扫描与血液采集,以获取DLPFC、VMPFC的T2信号值及血液白细胞(WBC)总数值,并进行比较;同时患者进行阳性与阴性症状量表(PANSS)评分;分析患者DLPFC、VMPFC的T2信号值、WBC总数及PANSS评分间的相关性。结果:患者组两侧DLPFC的T2信号强度、WBC总数明显高于对照组(t=2.57,2.35,2.16;P均<0.05)。患者组两侧DLPFC的T2信号强度与WBC总数呈正相关(r=0.21,0.36,P均<0.05);两侧DLPFC的T2信号强度、WBC总数与PANSS阴性症状分呈正相关(r=0.38,0.35,0.41;P均<0.05)。结论:首发精神分裂症患者DLPFC的T2信号强度与外周血WBC水平异常,提示炎症反应是精神分裂症发病的机制之一。

The precursor frequency of alloreactive CTLs is proportional to the number of T cell epitope specificities

The aim of this study is to find the experimental evidence that the precursor frequency of alloreactive CTLs is proportional to the number of the T-cell epitope specificities. The number of T-cell epitope specificities was manipulated by pulsing different humor of HLA-A2 restricted peptide（s） onto the T2 cells, which acted as stimulating cells to elicit allo-reaction by co-culturing with peripheral blood lymphocytes （PBLs） of HLA-A2 negative individual. Ten HLA-A2 restricted peptides （all were normal cell components ） were synthesized, and cell peptide extract was prepared by frozen and thawed. T2 cells loaded with different number of peptide（s） were co-cultured with PBLs of an HLA-A2 negative individual; the latter were stained with PKH67 in advance. Then the proliferation was monitored with flow cytometry, and the precursor frequency of the effector cells was ＇analyzed by the ModFit Software. After 6 d of culture, no proliferation was observed in the bulk culture of PBL alone, and obvious proliferation took place when PBLs of the HLA-A2 negative were co-cultured with T2 cells loaded with or without loading peptide（ s）. The precursor frequency of the alloreactive CTLs was 0.052 819 for co-culture with T2 cells loaded without peptide; however it was 0. 030 429 for T2 cells with EBV/LMP2A and 0. 030 528 for T2 cells loaded with a single autogeneic peptide, and increased up to 0. 144 942 for T2 cells loaded with 10 autogeneic peptides; the precursor frequency was 0. 203 649 when co-cultured with T2 cells loaded with miscellaneous peptides extracted from the cytoplasm of T2 cells. This study reveals that the precursor frequency of alloreactive CTLs is proportional to the number of T-cell epitope specificities, and independent of the density of the allogeneic HLA Class Ⅰ molecule. Our findings support the hypothesis that the alloreactive T cell populations comprise miscellaneous T cell clones; each is specific to corresponding pMHC. The novel constellation of peptides presented by allogeneic MHC molecules makes thousands of different epitopes, which account for the exceptional high precursor frequency of alloreactive T cells.

Analysis of tumor-infiltrating gamma delta T cells in rectal cancer

AIM: To investigate the regulatory effect of Vδ1 T cells and the antitumor activity of Vδ2 T cells in rectal cancer.METHODS: Peripheral blood, tumor tissues and para-carcinoma tissues from 20 rectal cancer patients were collected. Naïve CD4 T cells from the peripheral blood of rectal cancer patients were purified by negative selection using a Naive CD4+ T Cell Isolation Kit II (Miltenyi Biotec). Tumor tissues and para-carcinoma tissues were minced into small pieces and digested in a triple enzyme mixture containing collagenase type IV, hyaluronidase, and deoxyribonuclease for 2 h at room temperature. After digestion, the cells were washed twice in RPMI1640 and cultured in RPMI1640 containing 10% human serum supplemented with L-glutamine and 2-mercaptoethanol and 1000 U/mL of IL-2 for the generation of T cells. Vδ1 T cells and Vδ2 T cells from tumor tissues and para-carcinoma tissues were expanded by anti-TCR γδ antibodies. The inhibitory effects of Vδ1 T cells on naïve CD4 T cells were analyzed using the CFSE method. The cytotoxicity of Vδ2 T cells on rectal cancer lines was determined by the LDH method.RESULTS: The percentage of Vδ1 T cells in rectal tumor tissues from rectal cancer patients was significantly increased, and positively correlated with the T stage. The percentage of Vδ2 T cells in rectal tumor tissues from rectal cancer patients was significantly decreased, and negatively correlated with the T stage. After culture for 14 d with 1 μg/mL anti-TCR γδ antibodies, the percentage of Vδ1 T cells from para-carcinoma tissues was 21.45% ± 4.64%, and the percentage of Vδ2 T cells was 38.64% ± 8.05%. After culture for 14 d, the percentage of Vδ1 T cells from rectal cancer tissues was 67.45% ± 11.75% and the percentage of Vδ2 T cells was 8.94% ± 2.85%. Tumor-infiltrating Vδ1 T cells had strong inhibitory effects, and tumor-infiltrating Vδ2 T cells showed strong cytolytic activity. The inhibitory effects of Vδ1 T cells from para-carcinoma tissues and from rectal cancer tissue were not significantly different. In addition, the cytolytic activities of Vδ2 T cells from para-carcinoma tissues and from rectal cancer tissues were not significantly different.CONCLUSION: A percentage imbalance in Vδ1 and Vδ2 T cells in rectal cancer patients may contribute to the development of rectal cancer.

Aberrant activation of nuclear factor of activated T cell 2 in lamina propria mononuclear cells in ulcerative colitis

AIM:To investigate the role of nuclear factor of activated T cell 2(NFAT2),the major NFAT protein in peripheral T cells,in sustained T cell activation and intractable inflammation in human ulcerative colitis(UC). METHODS:We used two-dimensional gel-electrophoresis, immunohistochemistry,double immunohistochemical staining,and confocal microscopy to inspect the expression of NFAT2 in 107,15,48 and 5 cases of UC, Crohn's disease(CD),non-specific colitis,and 5 healthy individuals,respectively. RESULTS:Up-regulation with profound nucleo- translocation/activation of NFAT2 of lamina propria mononuclear cells(LPMC)of colonic mucosa was found specifically in the affected colonic mucosa from patients with UC,as compared to CD or NC(P<0.001,Kruskal- Wallis test).Nucleo-translocation/activation of NFAT2 primarily occurred in CD8+T,but was less prominent in CD4+T cells or CD20+B cells.It was strongly associated with the disease activity,including endoscopic stage (τ=0.2145,P=0.0281)and histologic grade(τ=0.4167, P<0.001). CONCLUSION:We disclose for the first time the nucleo-translocation/activatin of NFAT2 in lamina propria mononuclear cells in ulcerative colitis.Activation of NFAT2 was specific for ulcerative colitis and highly associated with disease activity.Since activation of NFAT2is implicated in an auto-regulatory positive feedback loop of sustained T-cell activation and NFAT proteins play key roles in the calcium/calcineurin signaling pathways,our results not only provide new insights into the mechanism for sustained intractable inflammation,but also suggest the calcium-calcineurin/NFAT pathway as a new therapeutic target for ulcerative colitis.

All-transRetinoic Acid Regulates Th1/Th2 Balance in CD4+T cells When GATA-3 is Deficient

The essential effect of vitamin A on immune function occurs through various mechanisms including direct effect on ThloTh2 balance modulation. However, it is unclear whether or not vitamin A can regulate Thl-Th2 balance under a strong Thl-polarizing condition. Therefore, the purpose of our study was to examine the effect of vitamin A metabolite allotrans retinoic acid （ATRA） on ThloTh2 differentiation in CD4~ T cells under GATA-3 deficiency, which can induce Thl-polarizing condition. In the present study, GATA-3 deficiency T cells were induced by siRNA and checked by real-time quantitative PCR and western blot. GATA-3 deficiency CD4＋ T cells and normal CD4＋ T were treated for 48 h with or without ATRA.

Estradiol regulates T cell activation by influencing co-stimulatory molecules transcription

To investigate whether estradiol （E2） plays a role in cell-contact-dependent regulatory mechanism of T cell activation, we studied the role of E2 in regulating gene transcription of CTLA-4, ICOS, B7-1, B7-2 and B7h in vitro. The splenic cells of normal female BALB/c mice were activated by ConA. Then the cells were cultured with E2 （100 pg/ml or 50 ng/ml） for 24 h or 48 h, respectively. The cell proliferation was measured by MTF assay and the expression of the co-stimulatory molecules mRNA was examined by RT-PCR analysis. We found that E2 （100 pg/ml, physiological level） stimulated the acti- vated spleen cells proliferation; inhibited CTLA-4, ICOS, TGF-β and IL-10 gene transcription; promoted B7-1 and B7-2 gene transcription. E2 （50 ng/ml, pregnant level） inhibited the proliferation of the activated splenic cells; promoted CTLA-4, B7-1, IL-10 but inhibited B7-2 and TGF-β gene transcription. Therefore, we conclude that the effects of E2 on T cell activation are partially through its regulation on the co-stimulatory molecules. The co-stimulatory molecules are crucial components of the cell-contact dependent regulatory mechanism, and E2 may regulate T cell activation by this mechanism.

多模态磁共振成像纹理特征分析鉴别肝细胞癌与肝脏局灶性结节性增生

目的基于多模态磁共振成像纹理特征分析鉴别肝细胞癌(HCC)与肝脏局灶性结节性增生(FNH).方法回顾性分析解放军总医院海南医院2012-04至2022-06经病理确诊的38例肝细胞癌和14例肝脏局灶性结节性增生患者,分别对两组患者的横轴位磁共振T_(2)加权成像(T_(2)WI)及扩散加权成像(DWI)图像进行纹理特征分析,参数包括角二阶矩(ASM)、对比度(contrast)、自相关(correlation)、逆差距(IDM)、熵(entropy).采用Kolmogorov-Smirnov检验及Mann-Whitney检验比较两组间纹理特征参数差异,并应用多元回归分析法获得整体模型拟合中入选变量及其值,得到回归方程,最终选择受试者工作曲线分析评估HCC与FNH的诊断效能.结果基于DWI图像纹理特征参数证实FNH组ASM、correlation、IDM显著大于HCC组,而FNH组的contrast、entropy则显著小于HCC组.基于T_(2)WI图像纹理特征参数证实FNH组的ASM、correlation显著大于HCC组,而FNH组的contrast、IDM、entropy则显著小于HCC组.DWI组在整体模型拟合中入选变量是entropy、contrast和常量,得到回归方程Y=-1.621×entropy-0.031×contrast+12.410;T_(2)WI组、T_(2)WI联合DWI(T_(2)WI-DWI)组入选变量及其值均相同,入选变量为entropy和常量,得到回归方程Y=-2.595×entropy+16.419.DWI组受试者工作特征曲线下面积(0.945)最大.结论基于多模态磁共振成像的图像纹理特征分析可以有效鉴别HCC与FNH.

Survivin HLA-A2^+高亲和性CTL表位的预测及鉴定

目的:采用生物信息方法预测和鉴定survivin抗原HLA-A2+限制性CTL表位,为探索基于survivin的肿瘤免疫治疗奠定基础。方法:采用超基序法和量化基序法对靶抗原survivin HLA-A2+限制性CTL表位进行预测;选取得分>10的表位肽为候选对象,并进行人工合成。采用T2细胞,以HLA-A2结合实验和流式细胞术(FITC染色)检测候选CTL表位肽的结合亲和力[以荧光系数(fluorescence index,FI)表示];以HLA-A2解离实验和流式细胞术检测其结合稳定性[以复合物解离50%的时间DC50(dissociation complex50%)表示]。结果:预测到的候选survivinCTL表位肽分别是:20STFKNWPFL28(SV20-28)、23KNWPFLEGC31(SV23-31)、96LTLGEFLKL104(SV96-104)、6LPPAWQPFL14(SV6-14)、33CTPERMAEA41(SV33-41)、46CPTE-NEPDL54(SV46-54)、130KVRRAIEQL138(SV130-138)、37RMAEAGFIH45(SV37-45)、88SVKKQFEEL96(SV88-96)。亲和力分析显示:SV20-28、SV96-104、SV130-138、SV23-31的FI分别为8.61、6.88、5.89、3.81;SV33-41、SV6-14、SV46-54、SV37-45、SV88-96的FI分别为0.31、-0.29、-0.4、-0.16和-0.03;稳定性分析结果DC50为:SV20-28、SV96-104、SV130-138>8h;SV23-31为4～6h;SV6-14、SV33-41、SV88-96为2～4h;SV46-54、SV37-45为0～2h。结果提示,SV20-28、SV96-104、SV130-138为高亲和力表位肽,SV23-31为中等亲和力表位肽,SV33-41、SV6-14、SV46-54、SV37-45、SV88-96为低亲和力表位肽。结论:超基序法、量化基序法可快速有效地预测抗原表位,SV20-28、SV96-104、SV130-138有可能是survivin HLA-A2+CTL表位,可用于后续研究。

Tapasin对HLA-E细胞表面表达的影响

目的 :探索伴侣分子Tapasin对HLA E分子细胞表面表达的影响。方法 :体外构建HLA EcDNA的逆转录病毒表达载体 ,并通过感染的方法将其转入Tapasin阴性的T2细胞系 ,利用流式细胞术检测HLA E分子在靶细胞表面的表达情况。结果 :外源HLA E基因在Tapasin阴性的T2细胞表面获得表达 (74 13% ) ,而对照细胞及经空载体转染的T2细胞表面未检测到HLA E分子的表达。结论 :HLA E分子的细胞表面表达也存在TAP非依赖的方式。

多肽:N-乙酰氨基半乳糖转移酶2真核表达载体的构建及在SHG-44细胞的表达

目的 :为探讨O 糖基化在肿瘤发生发展及转移中的作用和功能 ,构建pcDNA3/ppGalNAc T2真核表达质粒并转染人神经胶质瘤细胞SHG 4 4。方法 :采用PCR技术从pDONR2 0 1 T2得到ppGalNAc T2全长编码序列 ,亚克隆至真核表达载体pcDNA 3 1,脂质体介导基因转染人神经胶质瘤细胞SHG 4 4细胞 ,采用RT PCR法检测重组质粒的表达。结果 :酶切图谱分析和基因测序证实pcDNA3 1 T2真核表达质粒构建成功。RT PCR显示转染细胞有T2的表达。结论 :成功构建了真核表达载体pcDNA3 1 T2 ,并成功转染入SHG 4 4细胞 ,为进一步研究ppGalNAcT2的功能奠定了基础。

人多肽:N-乙酰氨基半乳糖转移酶2基因反义RNA表达质粒的构建及克隆鉴定

目的:研究反义封闭ppGalNAc-T2基因表达对胃癌细胞GC7901细胞增殖以及肿瘤细胞生物学行为的影响,构建反义表达载体并转染胃癌细胞GC7901。方法:在对几种肿瘤细胞的ppGalNAc-T2基因的表达水平分析后,以高表达ppGalNAc-T2的人胃癌细胞GC7901的总RNA为模板,利用RTPCR方法扩增两段不同长度ppGalNAc-T2基因片段,构建反义表达载体并转染胃癌细胞GC7901,通过G418筛选,建立一系列旨在封闭胃癌细胞GC7901细胞ppGalNAc-T2基因表达的亚细胞克隆。通过荧光显微镜、RT-PCR技术手段检测封闭反义ppGalNAc-T2基因RNA表达。结果:ppGalNAc-T2反义表达质粒载体pEGFP-FDT2和pEGFPFX-T2经限制性酶切及部分序列分析证明基因已正确插入载体中,荧光显微镜及RTPCR显示转染成功。结论:成功构建了ppGalNAc-T2反义表达质粒载体,反义封闭ppGalNAc-T2基因表达后,胃癌细胞GC7901ppGalNAc-T2的含量明显降低,为进一步研究ppGalNAc-T2奠定了基础。