罗汉果苷V调控高糖状态巨噬细胞M1极化促进骨髓间充质干细胞的成骨分化

背景:糖尿病微环境会造成巨噬细胞过度M1极化,这种高糖炎症状态会抑制骨髓间充质干细胞的成骨分化,从而影响糖尿病骨缺损的愈合。研究表明罗汉果苷Ⅴ具有抗炎、抗氧化、降血糖的作用,但其能否调节高糖炎症状态下巨噬细胞M1极化及骨髓间充质干细胞的成骨分化尚不清楚。目的:探讨罗汉果苷Ⅴ在高糖炎症状态下调节巨噬细胞M1型极化对骨髓间充质干细胞成骨分化的影响。方法:构建糖尿病C57BL/6小鼠模型,从正常和糖尿病小鼠分离骨髓来源巨噬细胞,分别培养于低糖和高糖培养基。使用脂多糖和干扰素γ作为炎症刺激诱导骨髓来源巨噬细胞的M1型极化,同时以160,320,640μmol/L罗汉果苷Ⅴ干预,用流式细胞术检测F4/80^(+)CD86^(+)细胞比例,qRT-PCR检测诱导型一氧化氮合酶、白细胞介素1β、白细胞介素6的mRNA表达水平,ELISA检测骨髓来源巨噬细胞上清液中肿瘤坏死因子α水平。分离C57BL/6小鼠骨髓间充质干细胞,分别使用低糖或高糖成骨诱导液诱导成骨分化,添加M1型巨噬细胞条件培养基作为炎症刺激,以及320μmol/L罗汉果苷Ⅴ干预,成骨诱导14 d后采用qRT-PCR检测碱性磷酸酶、Runt相关因子2、骨钙素、骨桥蛋白的mRNA表达水平,成骨诱导21 d后进行茜素红染色及定量分析。结果与结论:①流式细胞术结果显示320,640μmol/L罗汉果苷Ⅴ组的F4/80^(+)CD86^(+)细胞比例明显低于高糖炎症对照组(P<0.05);②qRT-PCR结果显示160,320,640μmol/L罗汉果苷Ⅴ组的诱导型一氧化氮合酶、白细胞介素6的mRNA相对表达量较高糖炎症对照组显著降低(P<0.05),320,640μmol/L罗汉果苷Ⅴ组白细胞介素1β的mRNA相对表达量较高糖炎症对照组显著降低(P<0.05);③ELISA结果显示160,320,640μmol/L罗汉果苷Ⅴ组的肿瘤坏死因子α分泌水平较高糖炎症对照组显著降低(P<0.05);④320μmol/L罗汉果苷Ⅴ干预后,高糖炎症状态下骨髓间充质干细胞的钙盐沉积增加(P<0.05),且碱性磷酸酶、Runt相关因子2和骨桥蛋白的mRNA相对表达量增加(P<0.05)。结果表明,罗汉果苷Ⅴ可通过抑制高糖炎症状态下骨髓来源巨噬细胞的M1型极化及炎症因子表达,促进骨髓间充质干细胞的成骨分化。

M2型巨噬细胞衍生外泌体促进小胶质细胞M2型极化

背景:目前对于M2型巨噬细胞衍生外泌体的研究多集中于促进伤口愈合及成骨细胞的增殖和分化,而很少有研究关注其对小胶质细胞表型的调控作用。目的:探讨M2型巨噬细胞衍生外泌体对于小胶质细胞的表型调控作用及分子机制。方法:①提取骨髓原代巨噬细胞,用50 ng/m L白细胞介素4刺激巨噬细胞24 h促进巨噬细胞M2型极化,流式细胞术和细胞免疫荧光鉴定M2型巨噬细胞标志物CD206;②提取和鉴定M2型巨噬细胞衍生外泌体;③将小胶质细胞BV2随机分为3组:对照组、脂多糖组、治疗组,对照组不做处理,脂多糖组加入500 ng/m L脂多糖干预24 h,治疗组同时加入500 ng/m L脂多糖和25μg/m L M2型巨噬细胞衍生外泌体干预24 h,ELISA检测培养上清中肿瘤坏死因子α和白细胞介素10的分泌量,q RT-PCR检测细胞中诱导型一氧化氮合酶、精氨酸酶1、白细胞介素1β和白细胞介素10的m RNA表达,Western blot检测诱导型一氧化氮合酶、精氨酸酶1的蛋白表达以及核因子κB信号通路相关蛋白表达。结果与结论:①ELISA结果显示,与对照组相比,脂多糖组肿瘤坏死因子α分泌明显增多;与脂多糖组相比,治疗组肿瘤坏死因子α的分泌减少而白细胞介素10的分泌增多;②q RT-PCR结果显示,与对照组相比,脂多糖组白细胞介素1β、诱导型一氧化氮合酶m RNA表达升高;与脂多糖组相比,治疗组白细胞介素1β、诱导型一氧化氮合酶m RNA表达降低,白细胞介素10、精氨酸酶1 m RNA表达升高;③Western blot结果显示,与对照组相比,脂多糖组诱导型一氧化氮合酶蛋白表达升高;与脂多糖组相比,治疗组诱导型一氧化氮合酶蛋白表达降低,而精氨酸酶1蛋白表达升高;(4)与对照组相比,脂多糖组核因子κB信号通路中P65、p-IκB-α蛋白表达降低;与脂多糖组相比,治疗组P65、p-IκB-α蛋白表达升高。结果表明:M2型巨噬细胞衍生外泌体可以显著抑制脂多糖诱导小胶质细胞的炎症反应,促进抗炎因子白细胞介素10的表达,抑制促炎因子肿瘤坏死因子α、白细胞介素1β的表达,促进小胶质细胞表型由M1型向M2型极化,其机制可能与M2型巨噬细胞衍生外泌体抑制核因子κB信号通路激活有关。

Microglia:a promising therapeutic target in spinal cord injury

Microglia are present throughout the central nervous system and are vital in neural repair,nutrition,phagocytosis,immunological regulation,and maintaining neuronal function.In a healthy spinal cord,microglia are accountable for immune surveillance,however,when a spinal cord injury occurs,the microenvironment drastically changes,leading to glial scars and failed axonal regeneration.In this context,microglia vary their gene and protein expression during activation,and proliferation in reaction to the injury,influencing injury responses both favorably and unfavorably.A dynamic and multifaceted injury response is mediated by microglia,which interact directly with neurons,astrocytes,oligodendrocytes,and neural stem/progenitor cells.Despite a clear understanding of their essential nature and origin,the mechanisms of action and new functions of microglia in spinal cord injury require extensive research.This review summarizes current studies on microglial genesis,physiological function,and pathological state,highlights their crucial roles in spinal cord injury,and proposes microglia as a therapeutic target.

Investigating Müller glia reprogramming in mice: a retrospective of the last decade, and a look to the future

Müller glia,as prominent glial cells within the retina,plays a significant role in maintaining retinal homeostasis in both healthy and diseased states.In lower vertebrates like zebrafish,these cells assume responsibility for spontaneous retinal regeneration,wherein endogenous Müller glia undergo proliferation,transform into Müller glia-derived progenitor cells,and subsequently regenerate the entire retina with restored functionality.Conversely,Müller glia in the mouse and human retina exhibit limited neural reprogramming.Müller glia reprogramming is thus a promising strategy for treating neurodegenerative ocular disorders.Müller glia reprogramming in mice has been accomplished with remarkable success,through various technologies.Advancements in molecular,genetic,epigenetic,morphological,and physiological evaluations have made it easier to document and investigate the Müller glia programming process in mice.Nevertheless,there remain issues that hinder improving reprogramming efficiency and maturity.Thus,understanding the reprogramming mechanism is crucial toward exploring factors that will improve Müller glia reprogramming efficiency,and for developing novel Müller glia reprogramming strategies.This review describes recent progress in relatively successful Müller glia reprogramming strategies.It also provides a basis for developing new Müller glia reprogramming strategies in mice,including epigenetic remodeling,metabolic modulation,immune regulation,chemical small-molecules regulation,extracellular matrix remodeling,and cell-cell fusion,to achieve Müller glia reprogramming in mice.

Recombinant chitinase-3-like protein 1 alleviates learning and memory impairments via M2 microglia polarization in postoperative cognitive dysfunction mice

Postoperative cognitive dysfunction is a seve re complication of the central nervous system that occurs after anesthesia and surgery,and has received attention for its high incidence and effect on the quality of life of patients.To date,there are no viable treatment options for postoperative cognitive dysfunction.The identification of postoperative cognitive dysfunction hub genes could provide new research directions and therapeutic targets for future research.To identify the signaling mechanisms contributing to postoperative cognitive dysfunction,we first conducted Gene Ontology and Kyoto Encyclopedia of Genes and Genomes pathway enrichment analyses of the Gene Expression Omnibus GSE95426 dataset,which consists of mRNAs and long non-coding RNAs differentially expressed in mouse hippocampus3 days after tibial fracture.The dataset was enriched in genes associated with the biological process"regulation of immune cells,"of which Chill was identified as a hub gene.Therefore,we investigated the contribution of chitinase-3-like protein 1 protein expression changes to postoperative cognitive dysfunction in the mouse model of tibial fractu re surgery.Mice were intraperitoneally injected with vehicle or recombinant chitinase-3-like protein 124 hours post-surgery,and the injection groups were compared with untreated control mice for learning and memory capacities using the Y-maze and fear conditioning tests.In addition,protein expression levels of proinflammatory factors(interleukin-1βand inducible nitric oxide synthase),M2-type macrophage markers(CD206 and arginase-1),and cognition-related proteins(brain-derived neurotropic factor and phosphorylated NMDA receptor subunit NR2B)were measured in hippocampus by western blotting.Treatment with recombinant chitinase-3-like protein 1 prevented surgery-induced cognitive impairment,downregulated interleukin-1βand nducible nitric oxide synthase expression,and upregulated CD206,arginase-1,pNR2B,and brain-derived neurotropic factor expression compared with vehicle treatment.Intraperitoneal administration of the specific ERK inhibitor PD98059 diminished the effects of recombinant chitinase-3-like protein 1.Collectively,our findings suggest that recombinant chitinase-3-like protein 1 ameliorates surgery-induced cognitive decline by attenuating neuroinflammation via M2 microglial polarization in the hippocampus.Therefore,recombinant chitinase-3-like protein1 may have therapeutic potential fo r postoperative cognitive dysfunction.

Postnatal development of rat retina:a continuous observation and comparison between the organotypic retinal explant model and in vivo development

The organotypic retinal explant culture has been established for more than a decade and offers a range of unique advantages compared with in vivo experiments and cell cultures.However,the lack of systematic and continuous comparison between in vivo retinal development and the organotypic retinal explant culture makes this model controversial in postnatal retinal development studies.Thus,we aimed to verify the feasibility of using this model for postnatal retinal development studies by comparing it with the in vivo retina.In this study,we showed that postnatal retinal explants undergo normal development,and exhibit a consistent structure and timeline with retinas in vivo.Initially,we used SOX2 and PAX6 immunostaining to identify retinal progenitor cells.We then examined cell proliferation and migration by immunostaining with Ki-67 and doublecortin,respectively.Ki-67-and doublecortin-positive cells decreased in both in vivo and explants during postnatal retinogenesis,and exhibited a high degree of similarity in abundance and distribution between groups.Additionally,we used Ceh-10 homeodomain-containing homolog,glutamate-ammonia ligase(glutamine synthetase),neuronal nuclei,and ionized calcium-binding adapter molecule 1 immunostaining to examine the emergence of bipolar cells,Müller glia,mature neurons,and microglia,respectively.The timing and spatial patterns of the emergence of these cell types were remarkably consistent between in vivo and explant retinas.Our study showed that the organotypic retinal explant culture model had a high degree of consistency with the progression of in vivo early postnatal retina development.The findings confirm the accuracy and credibility of this model and support its use for long-term,systematic,and continuous observation.

Müller cells are activated in response to retinal outer nuclear layer degeneration in rats subjected to simulated weightlessness conditions

A microgravity environment has been shown to cause ocular damage and affect visual acuity,but the underlying mechanisms remain unclear.Therefore,we established an animal model of weightlessness via tail suspension to examine the pathological changes and molecular mechanisms of retinal damage under microgravity.After 4 weeks of tail suspension,there were no notable alterations in retinal function and morphology,while after 8 weeks of tail suspension,significant reductions in retinal function were observed,and the outer nuclear layer was thinner,with abundant apoptotic cells.To investigate the mechanism underlying the degenerative changes that occurred in the outer nuclear layer of the retina,proteomics was used to analyze differentially expressed proteins in rat retinas after 8 weeks of tail suspension.The results showed that the expression levels of fibroblast growth factor 2(also known as basic fibroblast growth factor)and glial fibrillary acidic protein,which are closely related to Müller cell activation,were significantly upregulated.In addition,Müller cell regeneration and Müller cell gliosis were observed after 4 and 8 weeks,respectively,of simulated weightlessness.These findings indicate that Müller cells play an important regulatory role in retinal outer nuclear layer degeneration during weightlessness.

The cGAS-STING-interferon regulatory factor 7 pathway regulates neuroinflammation in Parkinson's disease

Interferon regulatory factor 7 plays a crucial role in the innate immune response.However,whether interferon regulatory factor 7-mediated signaling contributes to Parkinson's disease remains unknown.Here we report that interferon regulatory factor 7 is markedly up-regulated in a 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine-induced mouse model of Parkinson's disease and co-localizes with microglial cells.Both the selective cyclic guanosine monophosphate adenosine monophosphate synthase inhibitor RU.521 and the stimulator of interferon genes inhibitor H151 effectively suppressed interferon regulatory factor 7 activation in BV2 microglia exposed to 1-methyl-4-phenylpyridinium and inhibited transformation of mouse BV2 microglia into the neurotoxic M1 phenotype.In addition,si RNA-mediated knockdown of interferon regulatory factor 7 expression in BV2 microglia reduced the expression of inducible nitric oxide synthase,tumor necrosis factorα,CD16,CD32,and CD86 and increased the expression of the anti-inflammatory markers ARG1 and YM1.Taken together,our findings indicate that the cyclic guanosine monophosphate adenosine monophosphate synthase-stimulator of interferon genes-interferon regulatory factor 7 pathway plays a crucial role in the pathogenesis of Parkinson's disease.

过表达lncRNAHEM2M改善非酒精性脂肪肝病小鼠的肝脏损伤

目的探讨过表达长链非编码RNA(lncRNA)HEM2M对非酒精性脂肪肝病(NAFLD)小鼠肝损伤的影响。方法野生型C57BL/6(WT)和条件性髓系细胞lncRNAHEM2M过表达(MYKI)小鼠分别喂饲普通饮食(ND)和高脂饮食(HFD),即为WT+ND、MYKI+ND、WT+HFD和MYKI+HFD组。12周后行腹腔糖耐量及胰岛素耐量试验后处死小鼠,检测小鼠血清和肝脏组织的肝功能指标,制备肝脏组织切片后行HE染色和F4/80免疫组化染色,ELISA法检测肝脏组织中IL-6、IL-1β和TNF-α水平,qRT-PCR检测M1型(TNF-α、iNOS和IL-6)和M2型(Arg-1、YM-1和IL-10)巨噬细胞标志物mRNA表达,免疫印迹检测肝脏组织中P-AKT、T-AKT、NLRC4、caspase-1和GSDMD蛋白表达,比色法和免疫荧光测定肝脏组织caspase-1活性。结果与HFD喂饲的WT小鼠相比,MYKI+HFD小鼠肝功能损伤减轻(P<0.01),肝脏脂肪变缓解,肝脏巨噬细胞浸润减少,糖耐量损伤及胰岛素抵抗改善(P<0.01);MYKI+HFD小鼠肝脏组织IL-6、IL-1β和TNF-α水平降低(P<0.01),M1型巨噬细胞标志物mRNA表达减少(P<0.01),M2型mRNA表达增加(P<0.01);MYKI+HFD小鼠肝脏组织NLRC4炎症小体活性降低(P<0.01),活性caspase-1减少,GSDMD-N蛋白表达降低(P<0.05)。结论过表达lncRNAHEM2M降低NAFLD小鼠肝脏炎症因子水平,进而改善胰岛素抵抗并抑制肝脏NLRC4炎症小体激活,减少肝细胞焦亡,最终改善NAFLD小鼠肝脏损伤。

RBMX通过下调PKM2抑制膀胱癌细胞的增殖、迁移、侵袭和糖酵解

目的探讨X连锁RNA结合基序蛋白(RBMX)对膀胱癌细胞(1376细胞和UC-3细胞)的增殖、迁移、侵袭的影响以及其在糖酵解中的作用。方法采用慢病毒表达系统和siRNA干扰技术,分别构建RBMX过表达和敲低的膀胱癌细胞模型(1376细胞和UC-3细胞)。采用RT-qPCR和Westernblotting分别在mRNA水平和蛋白水平上检测细胞模型是否构建成功。通过EdU增殖实验和克隆形成实验检测过表达和敲低RBMX后细胞的生长和集落形成能力,同时通过Transwell实验分析过表达和敲低RBMX后对细胞迁移、侵袭能力的影响;随后,采用Westernblotting检测过表达和敲低RBMX后糖酵解关键蛋白PKM1(M1型丙酮酸激酶)和PKM2(M2型丙酮酸激酶)的表达变化;最后,利用葡萄糖和乳酸检测试剂盒分析过表达和敲低RBMX对膀胱癌细胞糖酵解的影响。结果RT-qPCR和Westernblotting结果显示,过表达RBMX膀胱癌细胞的mRNA和蛋白表达水平显著高于阴性对照组(P<0.05),敲低RBMX膀胱癌细胞的mRNA和蛋白表达水平显著低于阴性对照组(P<0.05)。过表达RBMX明显抑制膀胱癌细胞的增殖、克隆形成、迁移和侵袭,敲低RBMX则作用相反。Westernblotting实验结果显示,过表达RBMX使PKM1表达上升,PKM2表达下降,敲低RBMX则作用相反。葡萄糖消耗及乳酸生成实验表明,过表达RBMX均能抑制膀胱癌细胞葡萄糖消耗及乳酸生成(P<0.05),敲低RBMX均能促进膀胱癌细胞葡萄糖消耗及乳酸生成(P<0.05)。结论RBMX通过下调PKM2抑制膀胱癌的发生发展和糖酵解能力,有望成为膀胱癌诊断和治疗的潜在分子靶标。

下调METTL5通过Wnt/β-catenin信号通路抑制三阴乳腺癌细胞增殖、迁移与侵袭

目的探讨甲基转移酶5(methyltransferase-like 5,METTL5)在三阴乳腺癌(triple-negative breast cancer,TNBC)中的作用和潜在机制。方法采用免疫组织化学方法和Western blot检测TNBC肿瘤组织和细胞系中METTL5的表达情况。用靶向METTL5的shRNA(shRNA-METTL5)转染TNBC细胞后,用CCK-8、集落形成、伤口愈合以及Transwell实验分别检测细胞增殖活性、迁移与侵袭,Western blot检测Wnt/β-catenin信号关键蛋白的表达。构建异种移植瘤模型,验证敲降METTL5对TNBC细胞在体内生长以及Wnt/β-catenin信号活性的影响。结果METTL5在TNBC肿瘤组织和细胞系中表达上调(P<0.01)。敲降METTL5可抑制TNBC细胞的增殖、迁移和侵袭并降低了Wnt/β-catenin信号分子β-catenin、细胞周期蛋白(Cyclin)D1、基质金属蛋白酶(MMP)-2和MMP-7的表达(均P<0.01)。体内实验显示,敲降METTL5减缓了移植瘤生长和Wnt/β-catenin信号活性。结论敲降METTL5能抑制TNBC细胞的增殖、迁移与侵袭,其作用可能与抑制Wnt/β-catenin信号通路有关。

高速铁路主跨320 m钢-混部分斜拉桥无砟轨道适应性研究

南玉高铁六景郁江特大桥设计将钢-混部分斜拉桥结构引入时速350 km高速铁路领域,而300 m级以上大跨度桥上无砟轨道的竖向变形极易超限,影响列车通过的安全性和舒适性,因此,系统研究在此大跨桥梁结构上铺设无砟轨道的适应性十分必要。通过建立有限元及动力学模型,分析不同组合工况下无砟轨道结构的变形特点及动力特性,运用60 m弦测法探究各工况下无砟轨道的线形变化规律,从而确定大跨度钢-混部分斜拉桥铺设无砟轨道的适应性,并对设计和施工提出合理化建议。主要结论如下:在各种不利组合荷载作用下,桥上无砟轨道结构强度满足规范要求,列车通过大桥的各项安全性与舒适性指标均满足规范要求;混凝土收缩徐变和斜拉索升降温是影响无砟轨道线形标准的两大主因,应在无砟轨道施工前确保足够的沉降观测期和收缩徐变释放期,并充分考虑拉索的保温设计;在温度组合荷载作用下,桥上无砟轨道的60 m弦测不平顺幅值为6.79 mm,满足高速铁路静态验收标准;但在叠加列车荷载和收缩徐变后,变形弦测值均出现Ⅱ级及以上超限,通过合理设置预拱度后可有效改善轨道平顺性标准。

^(99m)TcO4-SPECT/CT甲状腺核素显像联合超声及TSH对甲状腺结节性质的诊断价值

目的通过高锝酸钠-单光子发射计算机断层显像/电子计算机X射线断层扫描技术(^(99m)TcO4-SPECT/CT)核素显像提供甲状腺结节功能状态、结节解剖特点以及超声检查联合血清促甲状腺激素(TSH)水平进一步鉴别诊断甲状腺结节的良恶性,客观评价甲状腺结节的良恶性情况,对甲状腺结节的良恶性做出早期诊断。方法对因甲状腺结节同时行^(99m)TcO4-SPECT/CT甲状腺核素显像、甲状腺B超及TSH水平检查的患者共80例(92个结节)进行回顾性分析,对比不同方法及联合检查对甲状腺结节的诊断效能。结果92个结节中良性74个,恶性18个;^(99m)TcO4-SPECT/CT甲状腺显像与超声检查比较灵敏度(77.8%)高,特异度(70.2%)及准确度(71.7%)低,假阳性率(29.7%)高,假阴性率(22.2%)低,两者之间灵敏度、特异度、准确度、假阳性率、假阴性率差异均具有统计学意义(P<0.05);两者准确度比较差异无统计学意义(P>0.05)。^(99)mTcO4-SPECT/CT甲状腺显像与超声检查比较灵敏度高,特异性及准确度低,假阳性率高,假阴性率低,两者之间灵敏度、特异度、准确度、假阳性率、假阴性率差异均具有统计学意义(P<0.05);两者准确度比较差异无统计学意义(P>0.05);^(99m)TcO4-SPECT/CT甲状腺显像与超声检查联合较单独核素、单独超声检查灵敏度(88.9%)、特异度(87.8%)、准确度(81.5%)高,假阳性率(12.1%)、假阴性率(11.1%)低;联合检查与单独核素特异度、准确度、假阳性率比较差异有统计学意义(P<0.05),灵敏度与假阴性率比较差异无统计学意义(P>0.05);联合检查与单独超声灵敏度、准确度、假阴性率比较差异有统计学意义(P<0.05);特异度与假阳性率比较差异无统计学意义(P>0.05)。结论超声可以作为甲状腺结节的首选检查方法,其特异性高,但灵敏度低。^(99m)TcO4-SPECT/CT甲状腺显像在提供功能和代谢信息的同时,能提供解剖信息;而血清TSH水平则可为甲状腺结节的良恶性鉴别提供重要的参考依据,尤其对于核素冷结节且超声实性结节的患者,更应参考其TSH水平,将三者结合起来判断甲状腺结节的性质,为临床提供恰当的治疗方案,这具有重要意义。

M-APSK鉴相算法与并行载波同步方法

为实现M进制幅相调制(M-APSK)体制下高阶调制信号的相位精细校正,将DVB-S2标准推荐的16APSK和32APSK的Q次方无数据辅助鉴相算法进行了扩展,以应用于64APSK、128APSK和256APSK等高阶调制。针对高阶调制的有效鉴相星座点占比较低时环路工作不稳定的问题提出了改进算法,通过对功率归一化后接收符号的幅值进行阈值判决,仅在高于阈值时进行鉴相,低于阈值时则不改变滤波器状态和相位补偿值,以提高星座点的鉴相有效性和可靠性,从而降低入锁门限。针对高速数传的符号速率非常高,而处理器的工作时钟频率相对较低的问题,提出了一种适用于M-APSK的并行载波同步方法,可以满足接收机工作时钟处理需要。相对于传统固定编码调制(CCM)的载波同步环路,该并行方法还可应用于可变编码调制(VCM)体制的频率跟踪。

贝伐珠单抗联合奥希替尼治疗伴EGFRT790M突变的晚期NSCLC的疗效观察

目的探讨伴表皮生长因子受体-T790M(EGFRT790M)突变的晚期非小细胞肺癌(NSCLC)应用贝伐珠单抗联合奥希替尼治疗的临床疗效。方法选取接受治疗并经病理检查证实伴EGFRT790M突变的晚期NSCLC患者102例进行研究。应用随机数字表法将上述患者分为对照组(n=51)与观察组(n=51)。对照组患者给予奥希替尼治疗,观察组患者给予贝伐珠单抗联合奥希替尼治疗,两组患者均治疗3个月。比较两组患者的近期疗效、远期疗效、血清指标[糖类抗原125(CA125)、癌胚抗原(CEA)、血管内皮生长因子(VEGF)]以及治疗过程中的不良反应。结果观察组患者治疗有效率为56.86%,高于对照组患者的治疗有效率(35.29%)(P<0.05);观察组患者有效控制率为88.24%,与对照组患者的有效控制率(78.43%)比较无统计学差异(P>0.05);观察组患者进展率为23.53%,低于对照组患者的进展率(47.06%)(P<0.05);观察组患者无进展生存期长于对照组患者(P<0.05);观察组患者病死率为9.80%,低于对照组患者病死率(31.37%)(P<0.05);治疗3个月后,观察组患者CA125、CEA、VEGF水平均低于对照组患者(P<0.05);治疗过程中,观察组不良反应率与对照组比较无统计学意义(P>0.05)。结论贝伐珠单抗联合奥希替尼治疗伴EGFRT790M突变的晚期NSCLC患者的临床疗效良好,可提高患者无进展生存期、降低肿瘤标志物表达水平。

m1A/m5C/m6A/m7G调控基因预测胃癌预后及免疫关联性

目的基于m1A/m5C/m6A/m7G甲基化调控基因建立胃癌预后风险预测模型,并分析该模型与免疫的关联性。方法通过癌症基因组图谱(TCGA)-胃癌数据集筛选表达具有显著差异的m1A/m5C/m6A/m7G调控基因,通过单基因Cox回归分析和LASSO算法构建预后风险评分(risk score,RS)模型,使用Kaplan-Meier(K-M)统计进行RS模型验证,并应用细胞系进行RT-qPCR验证。利用单因素、多因素Cox回归分析建立nomogram模型。使用CIBERSORT算法和estimate包进行免疫关联性分析。结果建立了基于八个甲基化调控基因的预后RS模型,将胃癌患者分为高风险和低风险。这八个基因在胃癌细胞系中高表达(P<0.05)。在TCGA-胃癌训练集和GSE62254-验证集中,患者总生存率(OS)与分组状态之间存在显著相关性(P<0.001)。nomogram生存模型预测的1年(C-index=0.703)、3年(C-index=0.729)和5年(C-index=0.734)生存率与实际生存率的一致性较好。免疫关联性分析表明,与低风险患者组相比,高风险患者组免疫评分和免疫检查点相关基因的表达较高(P<0.05)。结论基于m1A/m5C/m6A/m7G调控基因的预后RS模型可预测胃癌预后并指导个体免疫治疗决策。

压水堆核电厂一回路冷却剂条件110mAg胶体形成机理与制备研究

在模拟压水堆一回路冷却剂条件下,以硼锂溶液为介质、联氨还原硝酸银来制备胶体纳米银,并探究了还原剂、硼酸、Ag+浓度、温度与辐照条件对胶体银性能的影响。结果表明,加入硼酸与还原剂联氨可有效稳定胶体颗粒,联氨与银的摩尔比为1.0~2.0时Ag^(+)的还原率最高,胶体最稳定。随着银离子浓度升高,胶体颗粒表面负电荷增多,颗粒不易团聚,胶体稳定性增强。高温高压的水环境下,更易形成更大粒径的胶粒。辐照剂量在0.9 kGy~7.2 kGy范围内,在有无联氨的条件下均可形成胶体银。

青海门源M6.9级地震地表破裂特征及区域地震活动趋势分析

据中国地震台网正式测定,2022年1月8日1时45分青海海北州门源县发生6.9级地震,震源深度10 km。此次地震是2016年门源M6.4级地震之后冷龙岭地区再次发生强震活动。此次地震的宏观震中位于距门源县城浩门镇西北50 km的冷龙岭硫磺沟地区,并在硫磺沟—大西沟一带形成规模大且连续性较好的地表破裂。地表调查显示,同震地表破裂的总长度约为23 km,整体走向N40°~85°W,地表破裂主要由雁列的地震鼓包、张裂缝、剪切裂缝等形式组合而成,而且地表伴生了较多规模不等的滑坡、崩塌等次生地质灾害。根据地表破裂的规模、走向及破裂特点等,可将其分为3段:东段(硫磺沟段),长约10 km,走向N40°~60°W,破裂规模较小,以伴有重力作用的拉张裂缝为主;中段(道沟段),长约9 km,走向N70°W,破裂规模较大,以发育规模较大的地震鼓包和剪切裂缝为主,而且左旋位移较大;西段(大西沟段),长约4 km,走向N85°W,此段规模最小,以雁列的拉张裂缝为主。其中—东段一起组成了该破裂带的东支,而西段构成了西支,两者都具有明显的左旋走滑特征,并自东向西破裂整体呈左阶展布,在G227国道以东形成了具有拉张特征的左阶阶区。综合分析表明,此次,地震发生在祁连山块体的祁连-海原活动构造带,发震断裂应为海原左旋走滑断裂带的冷龙岭-托莱山断裂段。结合对祁连-海原构造带1900年以来强地震序列及托莱山断裂的初步研究认为,该构造带的历史地震活动整体具有不断向西发展的趋势,但在哈拉湖和托莱山之间存在较明显的地震空区,因而推断托莱山断裂未来的强震危险性有增强的可能。

m1A RNA甲基化对直肠腺癌的诊断效能分析

目的探索m1A相关基因表达和血浆m1A总体甲基化水平对直肠腺癌诊断和预后的预测价值。方法根据Sangerbox(基于TCGA和GTEx数据库)在线平台分析11个m1A甲基化相关基因在直肠腺癌中的差异表达,结合临床数据进行诊断效能和生存分析。同时,通过检测血浆m1A甲基化水平在直肠腺癌患者和正常人中差异情况,分析其对直肠腺癌的诊断价值。结果TRMT6,一种关键的m1A编码器基因,在不同病理状态的直肠腺癌中升高最为显著,并可作为直肠腺癌,特别是早期直肠腺癌的诊断标志物,其特异性和灵敏性高达82.86%和90.00%,而且TRMT6的高表达也预示着直肠腺癌预后较好(HR=0.22,95%CI:0.08~0.60,P=0.0014)。同时,血浆m1A甲基化水平在直肠腺癌相对于正常人显著性升高,对早期直肠腺癌有一定的诊断价值,其AUC约为0.8。结论m1A相关基因和血浆m1A甲基化在直肠腺癌中升高,可作为其潜在的早期诊断标志物。本研究为直肠腺癌早期诊断提供新的靶标,将有助于指导制定更有效的治疗策略。

西地那非通过促进巨噬细胞M2型极化缓解慢性盆腔疼痛大鼠痛觉和炎症

目的:探讨磷酸二酯酶5(PDE5)抑制剂西地那非对巨噬细胞极化介导的慢性盆腔疼痛痛觉和炎症的机制。方法:32只成年Wistar大鼠随机分为4组:Sham组、实验性自身免疫性前列腺炎(EAP)组、Sildenafil^(+)EAP组、MET^(+)Sildenafil^(+)EAP组,每组8只。皮下注射前列腺抗原(PAg)和弗氏完全佐剂诱导EAP模型,Sham组注射等量生理盐水,西地那非治疗EAP大鼠,另外,Sildenafil^(+)EAP处理基础上注射巨噬细胞M2型极化抑制剂二甲双胍。HE染色分析前列腺组织病理变化;von Frey纤维法检测大鼠盆腔痛觉反应率;ELISA检测血清细胞因子IL-10和TNF-α水平。流式细胞术检测血清iNOS^(+)和CD16/32^(+)巨噬细胞数量及CD206^(+)、CD10^(+)巨噬细胞数量。结果:与Sham组相比,EAP组前列腺腹侧腺体组织出现明显局灶性或多灶性炎症,盆腔痛觉反应率、血清炎症因子TNF-α水平、巨噬细胞M1型极化特征iNOS^(+)和CD16/32^(+)细胞数量显著升高(均P<0.05),而巨噬细胞M2型极化特征IL-10水平和CD206^(+)、CD10^(+)巨噬细胞数量显著减少(均P<0.05)。与EAP组相比,Sildenafil^(+)EAP组盆腔痛觉反应率、TNF-α水平、iNOS^(+)和CD16/32^(+)细胞数量显著降低(均P<0.05),而IL-10水平和CD206^(+)、CD10^(+)巨噬细胞数量显著升高(均P<0.05)。与Sildenafil^(+)EAP组相比,MET^(+)Sildenafil^(+)EAP组盆腔痛觉反应率、TNF-α水平、iNOS^(+)和CD16/32^(+)细胞数量显著升高(均P<0.05),而IL-10水平和CD206^(+)与CD10^(+)巨噬细胞数量显著降低(均P<0.05)。结论:PDE5抑制剂西地那非通过促进M2巨噬细胞极化阻断慢性盆腔疼痛和炎症。