左侧乳腺癌两种调强放射治疗计划剂量学比较

目的:比较左侧乳腺癌保乳术后两种调强放疗计划的剂量学差异,评价两种计划的剂量学特点,为临床治疗方法的优选提供依据。方法:选择8例左侧乳腺癌保乳术后患者,利用三维治疗计划系统为每例患者分别设计调强放射治疗计划(IMRT)和混合调强放射治疗计划(Hybrid IMRT)。在剂量体积直方图(DVH)上比较靶区和正常组织器官照射剂量、不均匀指数和适形指数。结果:在具有相同覆盖率(V95%)的情况下,Hybrid IMRT的靶区剂量均匀度优于IMRT。两种计划的适形指数,V105%,V110%,最大剂量(Dmax),最小剂量(Dmin),平均剂量(Dmean)均无显著差异。HybridIMRT和IMRT相比,同侧肺接受13Gy的体积(V13)由27.66%降至20.7%,对侧肺V5由8.01%降至2.25%;心脏V10,V20分别由35.23%,16.77%降至19.22%,10.6%;对侧乳腺V5,V10分别由35%,10.39%降至20.38%,5.7%,差异均具有统计学意义(P<0.05);而对于同侧肺V30,V40及心脏V40,分别升高了1.28%,1.48%,2.48%,差异有统计学意义(P<0.05)。结论:在乳腺癌患者放疗体位重复性不太好和(或)摆位精确性不能保证的情况下,混合调强放疗技术是更好的选择。

住院患者夜间睡眠质量及其影响因素的调查

目的了解住院患者夜间睡眠状况及其影响因素,并比较护理人员和患者关于住院患者夜间睡眠状况和影响因素的不同看法。方法采用匹兹堡睡眠质量指数(Pittsburgh sleep quality index,PSQI)量表和自行设计的住院患者夜间睡眠状况调查表(患者卷和护士卷)分别对397例患者(内科254例,外科143例)和101位夜班护士进行调查。结果在397例患者中,45.6%的住院患者存在睡眠质量问题。单因素分析结果显示:护士护理别的患者发出的声响、夜间治疗护理、电话铃声、空调发出的声音、护士交谈声、治疗仪器发出的声音、护士脚步声是干扰住院患者夜间睡眠的环境因素;疾病本身带来的不适、夜间起来上厕所、药物的夜间服用是生理及病理生理方面的影响因素;对病情的担心、情绪厌烦、想念亲人、难以自控等心理因素导致患者难以入睡。Logistic回归分析结果显示:影响住院患者夜间睡眠的因素包括对病情的担心、疾病本身带来的不舒适、夜间起来上厕所和护士的脚步声等。91.1%的护士能够意识到大部分住院患者的夜间睡眠状况较正常人差;患者和护士认为睡眠影响因素的排序在总体上比较一致,但在各自总体中所占的比例仍有较多项目存在统计学差异。结论大部分住院患者存在睡眠质量问题,其影响因素是多方面的;护理人员应从患者角度出发,系统了解住院患者的睡眠状况,采取个体化护理对策,改善住院患者的睡眠质量,促进其身心早日康复。

腺病毒E1A基因对人宫颈癌细胞体外增殖抑制的实验研究

目的:探讨聚已烯亚胺-四氧化三铁(PEI-Fe3O4)纳米粒E1A基因对人宫颈癌细胞体外增殖的抑制作用及其作用机制,为宫颈癌E1A基因治疗的可行性提供实验依据。方法:E1A基因经PEI-Fe3O4纳米粒载体介导转染人宫颈癌细胞(Hela细胞),用细胞计数法测绘生长曲线、计算倍增时间及软琼脂集落形成数目,观察E1A基因对该细胞系体外生长的影响。采用RT-PCR和Western印迹检测E1A基因在宫颈癌细胞中的表达及对HER-2/neu基因表达的影响。结果:转染E1A基因的人宫颈癌细胞系生长缓慢,倍增时间延长,是转染空载体组的1.53倍,是Hela细胞组的1.58倍;未经转染的Hela细胞系、转染空载体纳米粒的Hela细胞系(Hela-vect)及转染E1A基因的Hela细胞系(Hela-E1A),细胞集落形成率分别为30.48%,28.32%和6.62%,转染E1A基因组(Hela-vect)明显低于Hela和Hela-vect组(均P<0.05)。与Hela及Hela-vect组的集落形成率相比,Hela-E1A组集落形成抑制率分别为78.28%和76.62%。RT-PCR和Western印迹结果显示,E1A基因能在Hela细胞中稳定表达,且显著降低了HER-2/neu在宫颈癌细胞中的mRNA和蛋白表达水平。结论:PEI-Fe3O4纳米粒E1A基因能够明显抑制人宫颈癌细胞的生长,其作用机制可能与E1A抑制HER-2/neu基因的表达有关。

下调体外培养头颈部鳞状细胞癌细胞iASPP的表达能抑制细胞增殖、侵袭，增加对紫杉醇的化学敏感性（英文）

Objective Our previous study has revealed that iASPP is elevated in human head and neck squamous cell carcinoma(HNSCC)and iASPP overexpression signifcantly correlates with tumor malignant progression and poor survival of HNSCC.This study investigated the function of iASPP playing in proliferation and invasion of HNSCC in vitro.Methods HNSCC cell line Tu686 transfected with Lentiviral vector-mediated iASPP-specific shRNA and control shRNA were named the shRNA-iASPP group and shRNA-NC group,respectively.The non-infected Tu686 cells were named the CON group.CCK-8 assay,flow cytometry,transwell invasion assay were performed to detect the effects of iASPP inhibition in vitro.Results Our results demonstrated that the proliferation of shRNA-iASPP cells at the time of 72 h(F=32.459,P=0.000),96 h(F=51.407,P=0.000),120 h(F=35.125,P=0.000)post-transfection,was significantly lower than that of shRNANC cells and CON cells.The apoptosis ratio of shRNA-iASPP cells was 9.42%±0.39%(F=299.490,P=0.000),which was significantly higher than that of CON cells(2.80%±0.42%)and shRNA-NC cells(3.18%±0.28%).The percentage of shRNA-iASPP cells in G0/G1 phase was 74.65%±1.09%(F=388.901,P=0.000),which was strikingly increased,compared with that of CON cells(55.19%±1.02%)and shRNA-NC cells(54.62%±0.88%).The number of invading cells was 56±4 in the shRNA-iASPP group(F=84.965,P=0.000),which decreased significantly,compared with the CON group(111±3)and the shRNA-NC group(105±8).The survival rate of shRNA-iASPP cells administrated with paclitaxel was highly decreased,compared with CON cells and shRNA-NC cells(F=634.841,P=0.000).Conclusion These results suggest iASPP may play an important role in progression and aggressive behavior of HNSCC and may be an efficient chemotherapeutic target for the treatment of HNSCC.