XIVE种植体即刻植入即刻负重的临床观察

目的：评价XIVE种植体在上颌外伤前牙区即刻种植即刻负重修复的临床效果。方法：对26例前牙区单颗或多颗无法保留的外伤残根拔除后,即刻植入XIVE种植体,并即刻负重修复。种植体扭矩控制在35Ncm左右,初期稳定性良好。平均四到五个月后行永久修复。在植入后1、2、4个月对其进行临床及影像学检查。结果：32枚种植体有2枚种植体2周后出现松动,一个月后脱落,其余30枚均在预期时间内形成良好骨性愈合,最终完成修复。结论：上颌前牙区单颗或多颗牙外伤,残根无法保留者,行即刻种植即刻负重修复是可行。早期种植修复有利于减缓牙槽骨的吸收,保留软硬组织的形态,缩短疗程。     

基于供应链管理的CIO与CKO比较分析

通过对信息总监(chief information officer,CIO)和知识总监(chief knowledge officer, CKO)的职责比较务析,结合供应链管理(supply chain management,SCM)的需求与特点,分析在知识经济的背景下CIO和CKO在供应链管理中的作用。     

应用COⅠ基因序列探讨中国蚱总科四亚科部分物种的系统发生关系(英文)

通过测定蚱科26种蚱的线粒体DNA细胞色素c氧化酶Ⅰ基因的部分序列,分析了蚱亚科、短翼蚱亚科、刺翼蚱亚科及股沟蚱亚科部分物种的系统发育关系。以蜢总科的Vandiemenella viatica和Proriferasp.作为外群,构建了MP树和Bayes树。在获得的598bp的序列中,有289个变异位点,253个简约信息位点; A、T、G和C的碱基平均含量分别为31.6% ,32.7% ,19.5% ,16.2% , A+T含量高于G+C含量。分子系统树显示:蚱亚科尖顶蚱属和该亚科其他属的亲缘关系较远,而与短翼蚱亚科的狭顶蚱属有较近的亲缘关系。尖顶蚱属的广西尖顶蚱聚在短翼蚱科内,与该亚科的尖翅狭顶蚱形成姐妹群且支持两者关系的置信度很高,广西尖顶蚱不应属于蚱亚科尖顶蚱属。龙滩柯蚱与蚱属的桂南蚱形成姐妹关系,而庭蚱属的细庭蚱聚在柯蚱属中,且蚱亚科柯蚱属的防城柯蚱与刺翼蚱亚科的二刺羊角蚱形成姐妹关系,因此柯蚱属不是单系群,作为一个单独的属是可疑的;蚱属不是单系群,日本蚱也不是蚱属中的原始物种,锯齿股蚱和粗体蚱碱基序列完全相同,再次证明二者为同一物种。     

灯盏花产黄酮内生放线菌筛选及产黄酮能力的初步研究

通过黄酮类物质特异颜色反应和可见分光光度法,筛选产黄酮的灯盏花内生放线菌,研究灯盏花产黄酮内生放线菌在PDA、高氏1号和淀粉3种培养基上的产黄酮能力。结果表明:59株灯盏花内生放线菌中,8株菌的镁粉+浓盐酸、氯化铝、浓氨水3种颜色反应均成阳性,能够产生黄酮。形态学观察初步鉴定这8株菌均为链霉菌属(Streptomyces)。3种培养基中,在PDA培养基上灯盏花产黄酮内生放线菌的菌丝体生物量、黄酮含量和产量较高。8株灯盏花产黄酮内生放线菌中,菌株RA′1-7生长较好,菌株ELA′3-2和RA2-1菌丝体黄酮含量较高,菌株ELA′3-2菌丝体黄酮产量较高。     

Logistic模型预测东北越冬代水稻二化螟发生期

2001~2003年在吉林省柳河县绿色大米生产稻区,采用Logistic模型拟合越冬代二化螟Chilosuppressalis(Walker),有效积温和诱捕器诱蛾百分率的关系。结果表明logistic模型有较好的拟合性。由模型拟合结果预测当地越冬代二化螟发蛾始盛期、高峰期和盛末期所需有效积温分别为275.9,358.4和440.8日.度,可以适时指导大田防治。     

Increased CD45RA+ FoxP3(low) regulatory T cells with impaired suppressive function in patients with systemic lupus erythematosus

BACKGROUND: The role of naturally occurring regulatory T cells (Treg) in the control of the development of systemic lupus erythematosus (SLE) has not been well defined. Therefore, we dissect the phenotypically heterogeneous CD4(+)FoxP3(+) T cells into subpopulations during the dynamic SLE development. METHODLOGY/PRINCIPAL FINDINGS: To evaluate the proliferative and suppressive capacities of different CD4(+) T cell subgroups between active SLE patients and healthy donors, we employed CD45RA and CD25 as surface markers and carboxyfluorescein diacetatesuccinimidyl ester (CFSE) dilution assay. In addition, multiplex cytokines expression in active SLE patients was assessed using Luminex assay. Here, we showed a significant increase in the frequency of CD45RA(+)FoxP3(low) naive Treg cells (nTreg cells) and CD45RA(-)FoxP3(low) (non-Treg) cells in patients with active SLE. In active SLE patients, the increased proportions of CD45RA(+)FoxP3(low) nTreg cells were positively correlated with the disease based on SLE disease activity index (SLEDAI) and the status of serum anti-dsDNA antibodies. We found that the surface marker combination of CD25(+)CD45RA(+) can be used to defined CD45RA(+)FoxP3(low) nTreg cells for functional assays, wherein nTreg cells from active SLE patients demonstrated defective suppression function. A significant correlation was observed between inflammatory cytokines, such as IL-6, IL-12 and TNFα, and the frequency of nTreg cells. Furthermore, the CD45RA(+)FoxP3(low) nTreg cell subset increased when cultured with SLE serum compared to healthy donor serum, suggesting that the elevated inflammatory cytokines of SLE serum may promote nTreg cell proliferation/expansion. CONCLUSIONS/SIGNIFICANCE: Our results indicate that impaired numbers of functional CD45RA(+)FoxP3(low) naive Treg cell and CD45RA(-)FoxP3(low) non-suppressive T cell subsets in inflammatory conditions may contribute to SLE development. Therefore, analysis of subsets of FoxP3(+) T cells, using a combination of FoxP3, CD25 and CD45RA, rather than whole FoxP3(+) T cells, will help us to better understand the pathogenesis of SLE and may lead to the development of new therapeutic strategies.     

Determination of Baylisascaris schroederi Infection in Wild Giant Pandas by an Accurate and Sensitive PCR/CE-SSCP Method

It has been recognized that other than habitat loss, degradation and fragmentation, the infection of the roundworm Baylisascaris schroederi (B. schroederi) is one of the major causes of death in wild giant pandas. However, the prevalence and intensity of the parasite infection has been inconsistently reported through a method that uses sedimentation-floatation followed by a microscope examination. This method fails to accurately determine infection because there are many bamboo residues and/or few B. schroederi eggs in the examined fecal samples. In the present study, we adopted a method that uses PCR and capillary electrophoresis combined with a single-strand conformation polymorphism analysis (PCR/CE-SSCP) to detect B. schroederi infection in wild giant pandas at a nature reserve, and compared it to the traditional microscope approach. The PCR specifically amplified a single band of 279-bp from both fecal samples and positive controls, which was confirmed by sequence analysis to correspond to the mitochondrial COII gene of B. schroederi. Moreover, it was demonstrated that the amount of genomic DNA was linearly correlated with the peak area of the CE-SSCP analysis. Thus, our adopted method can reliably detect the infectious prevalence and intensity of B. schroederi in wild giant pandas. The prevalence of B. schroederi was found to be 54% in the 91 fecal samples examined, and 48% in the fecal samples of 31 identified individual giant pandas. Infectious intensities of the 91 fecal samples were detected to range from 2.8 to 959.2 units/gram, and from 4.8 to 959.2 units/gram in the fecal samples of the 31 identified giant pandas. For comparison, by using the traditional microscope method, the prevalence of B. schroederi was found to be only 33% in the 91 fecal samples, 32% in the fecal samples of the 31 identified giant pandas, and no reliable infectious intensity was observed.     

秋海棠属植物种质亲缘关系的ISSR分析

应用ISSR标记方法对秋海棠属(Begonia L.)植物33个种的种质亲缘关系进行分析,从70条引物中筛选出13个多态性引物,并通过POPgen 32软件以UPGMA法分析其亲缘关系。结果表明:33份秋海棠属植物的遗传距离在0.188 9～0.932 8之间,多态性百分率达到97.54%,Shannon信息指数为0.551 9,Nei基因多样性指数为0.376 0。秋海棠属植物具有丰富的遗传变异,UPGMA聚类分析结果与现有属下分类学表现较为一致,且生态地理条件相似的种群优先聚集。     

ABA对叶子花正常叶和变态叶部分生理生化指标的影响(研究简报)

为探索ABA对叶子花正常叶和变态叶部分生理生化指标的影响,利用不同浓度ABA溶液处理叶子花正常叶和变态叶,6h后,测定其叶绿素、可溶性糖、可溶性蛋白、游离脯氨酸含量和SOD酶活性.结果表明:处理后,变态叶和正常叶的叶绿素含量,SOD酶活性,游离脯氨酸含量和变态叶可溶性糖含量均先增加后降低,在ABA浓度为100 μmol/L时最大.正常叶的可溶性糖含量、正常叶和变态叶的可溶性蛋白含量在ABA浓度为50 μmol/L时最大.这表明50～100 μmol/L浓度的ABA能提高叶子花的抗逆性.     

父系HBeAg 阳性流产胚胎绒毛中HBV-DNA 的表达

目的:探讨在父系HBeAg阳性的流产胚胎中,乙型肝炎病毒在绒毛中的表达。方法:募集仅父系感染乙型肝炎病毒组合,即母HBsAg(-)且父HBsAg(+)流产胚胎。按以下组合将入选对象分为4组:组1为父HBeAg(+)母HBsAb(+);组2为父HBeAg(+)母HBsAb(-);组3为父HBeAg(-)母HBsAb(+);组4为父HBeAg(-)母HBsAb(-),采用酶联免疫吸附实验(ELISA)对胎儿父、母亲血清进行乙肝抗原、抗体检测,并使用荧光定量PCR法对胚胎绒毛进行HBV DNA检测。结果:父系感染乙型肝炎病毒的142例胚胎中,仅在父系HBeAg阳性组别(1、2组)84例胚胎中发现3例绒毛HBV-DNA升高,阳性率为3.57%。其中父HBeAg(+)母HBsAb(-)组合中2例,父HBeAg(+)母HBsAb(+)组合中1例。父系HBeAg均阳性,母系HBsAb阳性与阴性组间子代绒毛HBV-DNA升高率差异无显著性(P>0.05)。结论:HBeAg阳性父亲可能更容易导致乙肝父婴垂直传播。