^(99)Tc^m-MAG_3注射液的放射化学纯度分析

^(99)Tc^m-巯乙酰三甘氨酸(^(99)Tc^m-Mercaptoacetyltriglyeine,MAG_3)是目前^(99)Tc^m标记比较理想的肾小管分泌型显像剂。^(99)Tc^m-MAG_3注射液中可能含有未标记的高锝酸根(^(99)Tc^mO_4^-)、还原水解锝(H-R-^(99)Tc^m)等放射化学杂质,这些杂质直接影响显像的清晰程度。因此对^(99)Tc^m-MAG_3注射液的放射化学纯度(RCP)的分析是评价^(99)Tc^m-MAG_3注射液质量的重要指标之一。

哮喘中miR-29b、B7-H3调控巨噬细胞极化影响CD4^(+)T细胞分化的作用及机制研究

目的:探讨miR-29b、B7-H3调控巨噬细胞极化从而对CD4^(+)T分化产生影响的机制。方法:(1)收集在苏州大学附属儿童医院就诊的哮喘患儿及正常儿童外周血分离外周血单个核细胞(PBMC),提取RNA并进行逆转录,采用实时定量聚合酶链式反应(Q-PCR)技术测定miR-29b、B7-H3mRNA的表达,并收集患儿的哮喘家族史、变应性疾病史等。(2)THP-1细胞诱导为巨噬细胞后,用LV526、LV527和NC病毒侵染诱导成功的巨噬细胞形成miR-29b干扰、miR-29b过表达以及正常对照组,培养24 h后收集细胞检测STAT3和B7-H3基因及蛋白水平的表达。(3)验证STAT3为miR-29b的靶基因:接种THP-1细胞,加终浓度为50 ng/mL的PMA培养6 h后,换无PMA完全培养基继续培养24 h,然后用LV526、LV527和NC病毒侵染诱导成功的巨噬细胞形成miR-29b干扰、miR-29b过表达以及正常对照组,48 h进行荧光素酶分析来验证STAT3为miR-29b的靶基因。构建STAT3-3′-UTR荧光素酶报告基因质粒,并分为3组“miR-29b+STAT3-3′-UTR”、“miR-29b+STAT3-mut-3′-UTR”、“miR-29b+荧光素酶空载”。(4)不同处理方式的巨噬细胞与初始T细胞共培养3 d,Q-PCR检测T-bet、GATA3、ROR-γt的相对表达量。结果:(1)哮喘急性发作期组患儿的变应性疾病发生率高于其他两组(P=0.032),对照组的哮喘家族史远低于其他两组,差别具有统计学意义(P=0.001)。(2)哮喘急性发作期组PBMC中B7-H3表达量高于哮喘非急性发作期组与对照组,对照组PBMC中miR-29b表达量明显高于哮喘患儿非急性发作期组与急性发作期组(P<0.0001),哮喘非急性发作期组miR-29b表达量高于哮喘急性发作期组,差异有统计学意义(P=0.007)。(3)沉默表达miR-29b后巨噬细胞IL-4Rα、IL-4、IL-5、IL-13、CD206明显升高,而IFN-γ下降,提示miR-29b可以促进巨噬细胞向M2极化。(4)巨噬细胞过表达miR-29b,STAT3、B7-H3基因水平及蛋白水平表达下降;抑制miR-29b,STAT3、B7-H3基因水平及蛋白水平表达上升。(5)巨噬细胞STAT3与B7-H3mRNA的表达成显著正相关(r=0.9737,P<0.0001)。(6)STAT3是miR-29b的靶基因。(7)巨噬细胞与CD4^(+)T细胞共培养,可促进初始T细胞即Th0细胞向Th2方向分化,其中下调miR-29b的巨噬细胞促进作用更明显。结论:哮喘患儿PBMC中miR-29b表达量低于对照组儿童,而B7-H3高于对照组儿童,初步猜想miR-29b对于哮喘儿童具有保护作用,而B7-H3加重炎症反应。在巨噬细胞中下调miR-29b,可促进巨噬细胞向M2极化,巨噬细胞B7-H3及STAT3表达增加,使Th0细胞向Th2细胞分化,加重哮喘患者炎症反应。

Effect of macrophage polarization regulated by miR-29b,B7H3 on CD4^(+)T cell differentiation in asthma

Objective:To explore the mechanism that miR-29b and B7H3 regulate the polarization of macrophages and thus affect the differentiation of CD4^(+)T.Methods:1.PBMC was extracted from peripheral blood mononuclear cells of children with asthma and normal children in the affiliated Children's Hospital of Soochow University,and RNA was extracted and reverse transcribed.The expression of miR-29b and B7H3mRNA was determined by real-time quantitative polymerase chain reaction(Q-PCR).The family history of asthma and history of allergic diseases were collected.2.THP-1 cells were induced into macrophages,miR-29b interference,miR-29b overexpression and normal control were induced by LV526,LV527 and NC virus infection.After 24 hours of culture,the cells were collected to detect the expression of STAT3 and B7H3 genes and proteins.3.It was verified that STAT3 was the target gene of miR-29b:after inoculating THP-1 cells and culturing with PMA with final concentration of 50ng/ml for 6 hours,the macrophages without PMA were cultured for 24 hours,then the macrophages infected by LV528,LV529 and NC virus were induced to form miR-29b interference,miR29b overexpression and normal control group.Luciferase analysis was performed at 48 hours to verify that STAT3 was the target gene of miR-29b.STAT3-3'UTR luciferase reporter gene plasmids were constructed and divided into three groups:"miR-29b+STAT3-3'UTR","miR-29b+STAT3-mut-3'UTR"and"miR-29b+luciferase empty load".4.Macrophages with different treatments were co-cultured with initial T cells for 3 days.The relative expressions of T-bet,GATA3 and ROR-γt were detected by Q-PCR.Result:1.The incidence of allergic disease in the acute attack group(68%)was higher than that in the other two groups(34.8%,33.3%),and the family history of asthma in the normal group(0%)was much lower than that in the other two groups(52%,60.9%).The difference was statistically significant(P<0.05).2.The expression of B7H3 in PBMC in acute attack group was higher than that in non-acute attack group and normal group.The expression of miR-29b in PBMC in normal group was significantly higher than that in non-acute attack group and acute attack group(P<0.0001).The expression of miR-29b in non-acute attack group was significantly higher than that in acute attack group(P=0.007).3.After silencing the expression of miR-29b,IL-4Rα,IL-4,IL-5,IL-13 and CD206 of macrophages increased significantly,while IFN-γdecreased,suggesting that miR-29b can promote the polarization of macrophages to M2.4.The overexpression of miR-29b,STAT3 and B7H3 gene and protein level in macrophages decreased,while the increase of miR-29b,STAT3 and B7H3 gene and protein expression was inhibited.5.There was a significant positive correlation between the expression of STAT3 and B7H3mRNA in macrophages(r=0.9737,P<0.0001).6.STAT3 is the target gene of miR-29b.7.Co-culture of macrophages with CD4^(+)T cells can promote the differentiation of primary T cells,namely Th 0 cells,into Th2,and the promoting effect of macrophages with downregulation of miR-29b is more obvious.Conclusion:The expression of miR-29b in PBMC of children with asthma is lower than that of normal children,while the expression of B7H3 is higher than that of normal children.It is speculated that miR-29b has a protective effect on children with asthma,while B7H3 aggravates the inflammatory response.Down-regulation of miR-29b,in macrophages can promote macrophages to M2 polarization,increase the expression of B7H3 and STAT3 in macrophages,make Th0 cells differentiate into Th2 cells,and aggravate the inflammatory response in patients with asthma.

MgO-Al_(2)O_(3)-SiO_(2)玻璃的^(29)Si和^(27)Al固体核磁共振研究

铝硅酸盐玻璃具有高强度、硬度、弹性模量及良好的热学和化学稳定性,使其应用领域也越来越广泛。利用核磁共振(NMR)^(29)Si谱和^(27)Al谱,研究了不同Al/Si比MgO-Al_(2)O_(3)-SiO_(2)系玻璃的结构。研究表明,MgO-Al_(2)O_(3)-SiO_(2)系玻璃网络由硅氧网络和铝氧网络交替连接而成。由于游离氧不充足,大部分Al^(3+)都以5配位的形式存在于玻璃网络之外,只有25.0%~29.8%的Al^(3+)以[AlO_(4)]的形式存在,[AlO_(6)]的Al^(3+)其所占比例更少。随着Al/Si比例的增大,硅氧网络在镁铝硅玻璃结构中的聚合程度,呈现出了先增加而后降低的变化形式。在玻璃组分中Al与Si之间的比例为0.81时,由硅氧所形成的网络聚合程度达到极大值点。同时铝氧网络在玻璃结构中的聚合程度却呈现出了随Al/Si比的增加先是逐渐降低,在Al/Si=0.81时出现最小值。由[SiO_(4)]与[AlO_(4)]共同构成的整个玻璃网络的聚合程度呈现逐步降低的趋势。

重症肌无力患者外周血淋巴细胞表型的特点

用单或双染色免疫荧光技术经流式细胞仪分析，研究一组重症肌无力(MG）患者外周血淋巴细胞表型的表达。结果表明志者组CD16，56阳性(CD16，56)细胞百分率显著低于健康对照组(分别为9．92±6．88和18．08±8．02，P<0．05)。未经治疗的患者，CD3^+，CD29^+ CD4^+细胞百分旱和CD4／CD8比值均高于对照(依次为69．48±10．43．和60．80±12．35，32．88±5．90和25．77±4．38，1．79±0.84和1.39±0.44．P值均<0．05)。CD8^+及CD16，56^+细胞百分率均低于对照组(分别为22．47±7．09和29．26±8.64．8．80±5．50和18．08±8．02．P<0．05和P<0.01。胸腺摘除患者，CD3^+和CD8^+细胞百分旱与对照组无显著性差异，CD16．56^+、CD29^+ CD4^+细胞百分率及CD4／CD8比值均低于对照组(依次为P<0．05，P<0．01和P<0.05)。随访7例患者胸腺摘除术前、后淋巴细胞表型的变化，进一步显示手术后CD3^+、CD4^+.CD29^+CD4^+细胞和CD4／CD8比值下降．而CD8^+细胞百分率升高.