L形冷弯薄壁型钢组合钢管混凝土柱轴压性能

为解决异形钢管混凝土柱阴角对其承载力的影响,提出了用1个冷弯薄壁方钢管和2个U形钢管焊接成L形钢管,内填充混凝土形成L形冷弯薄壁型钢组合钢管混凝土柱形式。设计了5组共10根试件的轴压试验,并开展了有限元参数分析,研究了钢管厚度、U形管外伸长度和钢材强度等参数对构件承载力和延性等力学性能的影响。结果表明:该类试件的主要破坏形态为中上部局部鼓曲破坏,适量增大U形管外伸长度可以提高承载力,但增大到一定程度之后易发生弯扭破坏;承载力和延性随着钢管厚度和钢材强度增大而增加;混凝土强度对构件的初始刚度和峰值荷载的影响都很小,但对曲线下降段的影响较大;试件端部和中部截面阴角处的混凝土应力值比各边中部更大,说明采用U形钢管与方钢管组合的方式改善了阴角处钢管对混凝土约束普遍较弱的问题。基于“统一理论”,给出了两种承载力建议计算公式,与试验结果吻合较好,两种计算方法在0.44~1.94的约束效应系数范围内具有良好的适用性。

基于修正固有应变法的选区激光熔化成型316L钢块体残余应力预测

选区激光熔化(SLM)制造过程中极高的温度梯度及快速熔化凝固现象会在部件中产生复杂的残余应力分布,进而导致部件的变形、开裂,以及使用中的提前失效。因此,对SLM成型零件的残余应力预测至关重要。将修正固有应变(MIS)法用于SLM成型316L钢块体的残余应力预测。首先,采用热-力顺序耦合方法建立SLM成型的详细模型,从计算结果中提取固有应变并验证其准确性;随后,基于修正固有应变法建立10 mm×10 mm×10 mm的316L钢块体模型,模型由20个元层构成,每个元层中包含数个真实物理层;最后,通过逐层激活元层,并加载固有应变来模拟选区激光熔化成型过程,得到块体的应力-应变分布。以相同的工艺参数实际打印同尺寸的316L钢块体,使用X线衍射(XRD)法对块体的残余应力进行测量。结果表明:与XRD测量数据对比,修正固有应变法能够在较短时间内有效预测SLM成型316L钢块体的残余应力。

L形方钢管再生混凝土组合异形柱偏压承载力计算方法

基于叠加原理,在《矩形钢管混凝土组合异形柱技术规程》提供的理论计算公式基础上,研究了L形方钢管再生混凝土组合异形柱偏压承载力计算方法。在考虑再生混凝土有效约束面积影响的基础上,提出了L形方钢管再生混凝土组合异形柱偏压承载力计算公式,绘制出轴力-弯矩关系曲线。结果表明:通过引入钢管对内填再生混凝土的约束效应系数,考虑钢管对不同粗骨料取代率再生混凝土的有效约束作用,并根据约束强弱将钢管对内填再生混凝土的约束区域进行划分,可得到再生混凝土的有效约束面积;通过与试验及数值模拟结果对比,验证了L形方钢管再生混凝土组合异形柱偏压承载力计算公式的有效性,该公式可用于预测L形方钢管再生混凝土组合异形柱的偏压承载力,轴力-弯矩关系曲线可较为准确且安全地预测试件的承载力。

WC粒度配比对316L激光熔覆层耐磨/抗冲击性能的影响

目的通过调控熔覆层的凝固组织,在提升316L激光熔覆层耐磨性的同时,减小添加WC颗粒对冲击韧性的削弱。方法将316L粉末与WC颗粒球磨混合,采用激光熔覆技术,在316L钢基体表面制备3种质量分数为30%的不同WC粒度(75~150μm颗粒的WC(L)组,25~45μm颗粒的WC(S)组,混合粗细粒度颗粒的WC(L/S)组)增强的合金复合涂层。利用扫描电镜(SEM)、X射线衍射仪等对复合涂层的微观组织和物相进行分析,并使用摩擦磨损试验机和冲击韧性试验机测试室温下的摩擦磨损和冲击韧性。结果混合粒度WC颗粒在316L熔覆层中的使用能有效减少大粒径WC颗粒在凝固过程中的沉降现象,提升了颗粒分布均匀性,平均自由粒子间距离(λ)从WC(L)组的230μm减至WC(L/S)组的160μm,降低了30.43%。根据电子背散射衍射(EBSD)结果可知,WC颗粒及其分解产物在凝固过程中能够阻碍晶粒长大,并提供非均质形核点,从而细化晶粒。熔覆层的摩擦磨损性能随着WC颗粒粒度的变化而变化,WC(L/S)组熔覆层的磨损体积仅为无WC组的3.33%,WC(L)组体积损失率的76.60%,WC(S)组体积损失率的73.02%。混合粒度WC的使用降低了WC颗粒对熔覆层韧性的削弱,在相同质量分数下,WC(L/S)组熔覆层的冲击功分别为WC(L)组的104.86%,为WC(S)组的117.97%。结论在使用微米尺寸WC颗粒且质量分数均为30%时,WC颗粒的粒度配比对熔覆层的摩擦磨损性能和冲击韧性均有显著影响,其中粗、细混合的粒度配比是一种较好的选择。

BNIP3L介导的线粒体自噬在镉致大鼠大脑皮质神经元凋亡中的作用

为探究线粒体自噬受体Bcl-2/腺病毒E1B 19 kDa相互作用蛋白3样(BNIP3L)介导的线粒体自噬对镉致大鼠大脑皮质神经元凋亡的调控作用,利用RNA干扰技术建立大鼠大脑皮质神经元BNIP3L基因沉默模型,并经10μmol/L镉处理12 h,Western blot检测BNIP3L、帕金森氏蛋白2(Parkin)和线粒体凋亡通路相关蛋白cleaved caspase-9、cleaved caspase-3的表达水平,免疫荧光染色检测BNIP3L与线粒体标志蛋白TOMM20共定位,透射电镜检测细胞内线粒体自噬体数目,FITC Annexin V染色检测细胞凋亡水平。结果:大鼠大脑皮质神经元经镉处理12 h后,BNIP3L蛋白表达水平极显著升高(P<0.01),BNIP3L与TOMM20共定位增加,沉默BNIP3L极显著抑制镉致Parkin线粒体转位(P<0.01),抑制镉致细胞内线粒体自噬体形成,极显著促进镉致caspase-9、caspase-3激活和神经元凋亡(P<0.01)。结果表明,BNIP3L介导的线粒体自噬可抑制镉致大鼠大脑皮质神经元凋亡。

甘蓝型油菜BnaSLY1基因进化分析及功能研究

赤霉素调控植物表皮细胞增长、茎叶伸长以及株型建成。拟南芥SLY1属于F-box蛋白,它通过靶向泛素化赤霉素信号转导路径的负向调控因子——DELLA蛋白来影响植物生长发育,然而油菜中BnaSLY1的基因功能尚未揭示。本研究对BnaSLY1进行了表达特征和进化树分析,利用CRISPR/Cas9技术创制了BnaSLY1不同拷贝数的突变体,结合RNA-Seq技术对BnaSLY1的生物学功能及其对油菜生长发育的影响进行了研究。结果表明,甘蓝型油菜Westar中有2个SLY1同源拷贝BnaA01.SLY1和BnaA06.SLY1,它们表达模式基本相同,为组成型表达基因,其蛋白定位在细胞核,且在不同的油菜品种及十字花科植物间序列保守。与对照相比,单突bnaa01sly1和bnaa06sly1开花时间推迟,株高显著降低,而双突bnasly1还表现出深绿色光叶表型,叶片厚度增加,开花期比单突进一步推迟,株高也进一步降低。RNA-Seq结果显示,双突与Westar之间的差异表达基因显著富集在生长素信号转导路径以及蜡质合成通路,多个开花时间相关基因表达也发生显著变化。本研究表明, BnaSLY1除影响植物株高和开花时间等生长发育进程,还影响表皮蜡质合成,为探索赤霉素信号转导路径在甘蓝型油菜生长发育中的重要作用奠定了理论基础。

小麦穗粒数QTL分析及其对千粒重多效性评价

小麦穗粒数是典型的数量性状,与小麦产量密切相关。为进一步挖掘小麦穗粒数的数量性状位点(quantitative trait loci, QTL),本研究以扬麦4号/偃展1号衍生的151个重组自交系(recombinant inbred line, RIL)(F10)为材料,利用小麦55K单核苷酸多态性(single-nucleotide polymorphism, SNP)基因芯片构建高密度遗传图谱,结合3年4个环境的表型数据对穗粒数性状进行QTL定位分析。在染色体4A、5A和5B上共检测到3个与穗粒数相关的QTL。其中,QGns.yaas-4A和QGns.yaas-5B在2个环境中均能被检测到,增加穗粒数的效应都来源于扬麦4号,表型贡献率分别为11.50%~13.27%和5.59%~10.99%,物理区间分别为703.41~710.25 Mb和77.62~365.60 Mb;QGns.yaas-5A在4个环境中被检测到,增加穗粒数的效应来源于偃展1号,表型贡献率为8.99%~11.13%,物理区间为495.34~512.39Mb。分析定位结果发现,QGns.yaas-5A增加穗粒数的等位变异(YZ1等位变异)和QGns.yaas-5B上的增加穗粒数的等位变异(YM4等位变异)可显著增加千粒重,分别增效3.50%(P<0.05)和4.45%(P<0.01)。开发了QGns.yaas-4A、QGns.yaas-5A和QGns.yaas-5B的KASP (Kompetitive Allele-Specific PCR)标记,在自然群体中验证表明,聚合3个增加穗粒数等位变异的位点具有显著的加性效应,可增加13.75%的穗粒数。该研究结果为小麦穗粒数分子标记辅助育种提供理论和技术支撑。

缺血性脑卒中铁死亡特征基因NFE2L2的鉴定与验证

背景:铁死亡与缺血性脑卒中的发病密切相关,靶向铁死亡是一种治疗缺血性脑卒中有前景的方案,但具体调控靶点尚不明确。目的:通过生物信息学和机器学习方法筛选缺血性脑卒中铁死亡相关特征基因,并通过细胞实验进行验证,探讨铁死亡在缺血性脑卒中的作用。方法:基于GEO数据库和FerrDb数据库选取符合条件的缺血性脑卒中相关数据集和铁死亡表达数据集,通过t检验筛选铁死亡相关差异基因。对铁死亡相关差异基因进行GO功能富集分析与KEGG信号通路富集分析。通过PPI网络分析和机器学习筛选缺血性脑卒中铁死亡的特征基因,利用ROC分析和GSEA分析探究特征基因的准确性和生物功能。然后进行细胞实验,将HT22细胞分为对照组与缺血性脑卒中组,对照组不作任何干预,缺血性脑卒中组加入0.1 mol/L的H_(2)O_(2)干预24 h诱导细胞氧化应激和铁死亡,通过实时荧光定量RT-PCR和Western Blot验证铁死亡的发生和特征基因表达。结果与结论:(1)共获取45个铁死亡相关差异基因,GO和KEGG富集分析发现差异基因与氧化应激、自噬、铁死亡、脂肪细胞因子信号通路和线粒体代谢密切相关。(2)通过PPI网络中的MCODE插件和cytoHubba插件与机器学习中的LASSO算法和SVM-RFE算法共鉴定出1个铁死亡特征基因核因子E2相关因子2(nuclear factor erythroid 2-related factor 2,NFE2L2)。(3)对NFE2L2进行ROC曲线分析,发现在训练集和验证集中构建的诊断预测模型具有良好的准确性与特异性;对NFE2L2进行GSEA分析,发现特征基因通过免疫、炎症反应、氨基酸代谢及神经因子调控等方面参与缺血性脑卒中发病机制的调控。(4)细胞实验的RT-PCR和Western Blot分析表明,与对照组对比,缺血性脑卒中组中的酰基辅酶A合成酶长链家族成员4 mRNA和蛋白表达水平显著增高(P<0.05),谷胱甘肽过氧化物酶4 mRNA和蛋白表达水平显著降低(P<0.05);与对照组对比,缺血性脑卒中组中特征基因NFE2L2 mRNA和蛋白表达水平显著增高(P<0.05)。(5)上述结果证实,缺血性脑卒中与铁死亡密切相关,靶向特征基因NFE2L2可以为研究和治疗缺血性脑卒中提供一定的思路与方向。

基于整车关键尺寸L114的平台架构研究

为了研究最优的整车平台架构策略,本文详细阐述平台架构的概念,定义了架构关键尺寸L114,列举国内某车企基于关键尺寸L114一致的平台拓展尺寸链,并梳理该平台架构乘员舱架构件具体的策略,通过对比分别采取平台车型关键尺寸L113一致与平台车型关键尺寸L114一致时的平台通用化率,发现2种策略的平台通用化率基本一致。同时结合整车安全碰撞策略进行分析,结果表明,若采用关键尺寸L114更具优势,该策略下同平台车型仅需满足高车型的碰撞策略,即可同步满足其他车型的侧碰要求,有效降低平台开发成本。

Effects of P301L-TAU on post-translational modifications of microtubules in human iPSC-derived cortical neurons and TAU transgenic mice

TAU is a microtubule-associated protein that promotes microtubule assembly and stability in the axon.TAU is missorted and aggregated in an array of diseases known as tauopathies.Microtubules are essential for neuronal function and regulated via a complex set of post-translational modifications,changes of which affect microtubule stability and dynamics,microtubule interaction with other proteins and cellular structures,and mediate recruitment of microtubule-severing enzymes.As impairment of microtubule dynamics causes neuronal dysfunction,we hypothesize cognitive impairment in human disease to be impacted by impairment of microtubule dynamics.We therefore aimed to study the effects of a disease-causing mutation of TAU(P301L)on the levels and localization of microtubule post-translational modifications indicative of microtubule stability and dynamics,to assess whether P301L-TAU causes stability-changing modifications to microtubules.To investigate TAU localization,phosphorylation,and effects on tubulin post-translational modifications,we expressed wild-type or P301L-TAU in human MAPT-KO induced pluripotent stem cell-derived neurons(i Neurons)and studied TAU in neurons in the hippocampus of mice transgenic for human P301L-TAU(p R5 mice).Human neurons expressing the longest TAU isoform(2N4R)with the P301L mutation showed increased TAU phosphorylation at the AT8,but not the p-Ser-262 epitope,and increased polyglutamylation and acetylation of microtubules compared with endogenous TAU-expressing neurons.P301L-TAU showed pronounced somatodendritic presence,but also successful axonal enrichment and a similar axodendritic distribution comparable to exogenously expressed 2N4R-wildtype-TAU.P301L-TAU-expressing hippocampal neurons in transgenic mice showed prominent missorting and tauopathy-typical AT8-phosphorylation of TAU and increased polyglutamylation,but reduced acetylation,of microtubules compared with non-transgenic littermates.In sum,P301L-TAU results in changes in microtubule PTMs,suggestive of impairment of microtubule stability.This is accompanied by missorting and aggregation of TAU in mice but not in i Neurons.Microtubule PTMs/impairment may be of key importance in tauopathies.

λ-Red重组技术结合复合诱变提高大肠杆菌L-异亮氨酸合成能力

本研究旨在通过λ-Red重组技术结合复合诱变方法提高大肠杆菌L-异亮氨酸合成能力。以E. coli NXA为出发菌株,首先采用λ-Red同源重组敲除编码支链氨基酸转运蛋白基因brnQ,获得突变菌株E. coli NXA1。然后将E. coli NXA1经常温常压等离子体(ARTP)、紫外(UV)与亚硝基胍(NTG)多轮复合诱变,以α-氨基丁酸(α-AB)为结构类似物进行筛选,筛选得到突变菌株E. coli NXA2。摇瓶发酵结果表明,在37℃、200 r/min条件下发酵40 h后,E. coli NXA1的L-异亮氨酸滴度为2.76 g/L,较E. coli NXA提高了33.98%;E. coli NXA2的L-异亮氨酸滴度为3.22 g/L,较E. coli NXA1提高了16.67%,较E. coli NXA提高了56.31%。对菌株E. coli NXA2经连续传代20代后,表现出较好的遗传稳定性。λ-Red重组技术结合复合诱变对大肠杆菌提高L-异亮氨酸合成能力有明显效果,为选育L-异亮氨酸高产菌株奠定理论基础。

多黏类芽孢杆菌Paenibacillus polymyxa ZJ-9芽孢萌发条件与过程的研究

多黏类芽孢杆菌(Paenibacillus polymyxa)具有抗病促生能力,在农业上得到广泛应用,芽孢特殊的抗逆性使得其方便运输和贮存,但自然条件下P.polymyxa萌发率低,限制了其推广应用。本文研究了P.polymyxa ZJ-9芽孢的热激活条件和萌发工艺,对萌发过程进行了表征。结果表明:在75℃、30 min的热激活条件下,芽孢的存活率达到98%以上且仍有较高的萌发水平;采用溶解于磷酸盐缓冲液(PBS)的L-丙氨酸+蔗糖(10.0 mmol/L)混合溶液,在室温恒温萌发12 h后,萌发率达到63.9%。对萌发过程表征发现,添加L-丙氨酸使得芽孢内2,6-吡啶二羧酸钙(DPA-Ca^(2+))释放量提高了3.35倍,利用透射电子显微镜(TEM)观察到芽孢复水现象增强,可见L-丙氨酸对芽孢萌发有明显促进作用。本研究为P.polymyxa芽孢制剂的应用提供了有益思路。

关于L-代数中理想的一些注记

许多逻辑代数可以看成L-代数.讨论一些特殊的L-代数,给出其L-理想与格滤子之间的关系.刻画一类使得L-理想集与格滤子集相等的格L-代数,同时给出L-代数与蕴含格之间的一个等价刻画.进一步给出格序效应代数的理想与L-理想以及它的同余与L-同余的等价刻画.

不同焊丝激光-MIG复合焊接SUS301L/Q450NQR1异种钢接头的组织及性能

为了降低成本,采用ER309LSi和CHW-55CNH两种不同焊丝,利用激光-MIG复合焊对Q450NQR1和SUS301L钢板进行对接焊,对比研究了两种焊丝接头的组织与性能。结果表明:两种焊丝接头均无未焊透、未熔合等缺陷,焊缝表面呈明显的鱼鳞纹;ER309LSi焊丝接头焊缝中心区主要为树枝状结晶的奥氏体以及少量铁素体组成;CHW-55CNH焊丝接头焊缝中心区主要由先共析铁素体以和珠光体组成;CHW-55CNH焊丝接头焊缝硬度(374 HV)大于ER309LSi焊丝接头(217 HV);ER309LSi焊丝接头平均抗拉强度(632.3 MPa)略大于CHW-55CNH焊丝接头(608.6 MPa);两种焊丝接头的中性盐雾腐蚀试验结果相差不大,电化学分析试验结果表明ER309LSi焊丝接头的耐蚀性优于CHW-55CNH焊丝接头。综上,当构件受力或耐蚀性要求不严格的时候,可以用价格较低的CHW-55CNH焊丝替代ER309LSi焊丝。

载富血小板血浆水凝胶对L929细胞氧化损伤的保护作用

背景:在慢性创面愈合过程中,活性氧的过量生成可能会损害L929成纤维细胞的功能,从而延缓创面修复,因此保护成纤维细胞免受氧化应激的影响对于促进创面愈合非常重要。目的:评估羧甲基壳聚糖-氧化硫酸软骨素/富血小板血浆(CMC-OCS/PRP)水凝胶对H2O2刺激下L929细胞的保护作用。方法:制备CMC-OCS/PRP水凝胶,表征水凝胶的微观形貌、降解性能、清除H2O2与羟基自由基的能力及生物相容性。取生长状态良好的L929细胞,分5组培养:对照组常规培养,H2O2组加入H2O2,CMC-OCS组加入羧甲基壳聚糖-氧化硫酸软骨素水凝胶浸提液+H2O2,PRP组加入富血小板血浆凝胶浸提液+H2O2,CMC-OCS/PRP组加入羧甲基壳聚糖-氧化硫酸软骨素/富血小板血浆水凝胶浸提液处理+H2O2,每组先加入水凝胶浸提液处理6 h,然后再加入H2O2处理24 h。培养结束后,检测细胞活性氧及丙二醛水平,细胞凋亡、胶原纤维Ⅰ蛋白表达。在加入H2O2的情况下,将上述水凝胶浸提液分别与L929成纤维细胞直接或间接共培养36 h,通过划痕实验、Transwell小室实验检测细胞的迁移能力。结果与结论:①CMC-OCS/PRP水凝胶具有均匀相互关联的多孔结构及良好的降解能力,体外可有效清除H2O2与羟基自由基,并且具有良好的生物相容性;②与对照组比较,H2O2组细胞凋亡率、细胞活性氧与丙二醛水平升高(P<0.05),细胞铺展面积减少(P<0.05),胶原纤维Ⅰ蛋白表达无明显变化(P>0.05);与H2O2组比较,CMC-OCS组、CMC-OCS/PRP组细胞活性氧水平降低(P<0.05),PRP组、CMC-OCS组、CMCOCS/PRP组丙二醛水平降低(P<0.05)、细胞铺展面积增加(P<0.05),CMC-OCS/PRP组细胞凋亡率降低(P<0.05),PRP组、CMC-OCS组、CMCOCS/PRP组胶原纤维Ⅰ蛋白表达增加(P<0.05);③与对照组比较,H2O2组细胞迁移数量减少(P<0.05),迁移面积无明显变化(P>0.05);与H2O2组比较,PRP组、CMC-OCS组、CMC-OCS/PRP组细胞迁移数量、迁移面积均增加(P<0.05),并且以CMC-OCS/PRP组增加最显著;④在氧化应激条件下,CMC-OCS/PRP水凝胶可改善成纤维细胞的迁移能力,抗细胞凋亡并保护细胞伸展功能。

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.

核电用316L不锈钢中厚板焊接工艺研究

某核电真空室项目主要采用316L不锈钢材料制造,根据零件结构特点,制造过程存在大量要求单面焊双面成形的焊缝,且所有焊缝均要求全熔透,同时焊缝磁导率≤1.03H/m,整体轮廓度±3mm,制造难度非常大。基于上述情况,决定进行专项科研立项攻关和研究,最终决定采用激光焊(打底)+TIG焊(填充)的焊接方法,采取理论分析与试验相结合的方式。通过对厚度为40mm中厚板进行相应的焊接工艺研究,确保焊接方法和工艺完全满足实际工程设备的需要,为项目的推进做好充分准备。

Autism spectrum disorder:difficulties in diagnosis and microRNA biomarkers

We performed a PubMed search for microRNAs in autism spectrum disorder that could serve as diagnostic biomarkers in patients and selected 17 articles published from January 2008 to December 2023,of which 4 studies were performed with whole blood,4 with blood plasma,5 with blood serum,1 with serum neural cell adhesion molecule L1-captured extracellular vesicles,1 with blood cells,and 2 with peripheral blood mononuclear cells.Most of the studies involved children and the study cohorts were largely males.Many of the studies had performed microRNA sequencing or quantitative polymerase chain reaction assays to measure microRNA expression.Only five studies had used real-time polymerase chain reaction assay to validate microRNA expression in autism spectrum disorder subjects compared to controls.The microRNAs that were validated in these studies may be considered as potential candidate biomarkers for autism spectrum disorder and include miR-500a-5p,-197-5p,-424-5p,-664a-3p,-365a-3p,-619-5p,-664a-3p,-3135a,-328-3p,and-500a-5p in blood plasma and miR-151a-3p,-181b-5p,-320a,-328,-433,-489,-572,-663a,-101-3p,-106b-5p,-19b-3p,-195-5p,and-130a-3p in blood serum of children,and miR-15b-5p and-6126 in whole blood of adults.Several important limitations were identified in the studies reviewed,and need to be taken into account in future studies.Further studies are warranted with children and adults having different levels of autism spectrum disorder severity and consideration should be given to using animal models of autism spectrum disorder to investigate the effects of suppressing or overexpressing specific microRNAs as a novel therapy.

慈姑多糖调控TLR4/MyD88/NF-κB抑制细胞炎症和氧化损伤对多种重金属诱导L02肝细胞凋亡的影响

目的探索慈姑多糖(Sagittaria Sagittifolia polysaccharide,SSP)是否通过介导Toll样受体4(Toll-like receptors 4,TLR4)/髓样分化因子88(myeloid differentiation factor 88,MyD88)/核转录因子-κB(nuclear transcription factor-kappa B,NF-κB)信号通路对6种重金属联合所致L02肝细胞损伤发挥保护作用。方法首先根据北京市售大米6种重金属膳食摄入比例,构建6种重金属混合染毒液所致L02细胞损伤体外模型。应用MTT法检测不同质量浓度慈姑多糖(0.25、0.5、1、2 mg/mL)提前作用24 h对L02细胞存活率的影响;Annexin V-FITC/碘化丙啶(PI)双染流式结合Hoechst 33342荧光检测细胞凋亡;DCFH-DA荧光探针检测细胞中活性氧(reactive oxygen species,ROS)含量变化;Western blot法检测细胞中多聚ADP核糖聚合酶1(poly-ADP ribose polymerase1,PARP1)、动力相关蛋白1(dynamin-related protein 1,Drp1)、肿瘤坏死因子-α(tumor necrosis factor-α,TNF-α)、白介素(interleukin,IL)-1β、IL-17、TLR4、MyD88、NF-κB p65蛋白表达情况。结果MTT结果显示,SSP在1 mg/mL作用24 h保护效果最佳;与模型组相比,SSP治疗组中ROS含量及细胞凋亡率均明显下降(P<0.05),Drp1、TNF-α、IL-1β、IL-17和TLR4、MyD88、NF-κB p65蛋白表达均显著降低(P<0.05),PARP1蛋白表达显著升高(P<0.01)。结论SSP可有效改善6种重金属联用诱导的L02细胞凋亡,可能与调控TLR4/MyD88/NF-κB信号通路抑制氧化损伤和炎症反应相关。

Melon2K array:A versatile 2K liquid SNP chip for melon genetics and breeding

High-throughput genotyping tools can effectively promote molecular breeding in crops.In this study,genotyping by target sequencing(GBTS)system was utilized to develop a genome-wide liquid SNP chip for facilitating genetics and breeding in melon(Cucumis melo L.),a globally cultivated economically important horticultural crop.Based on over eight million SNPs derived from 823 representative melon accessions,16K,8K,4K,2K,1K,500,250 and 125 informative SNPs were screened and evaluated for their polymorphisms,conservation of flanking sequences,and distributions.The set of 2K SNPs was found to be optimal for representing the maximum diversity with the lowest number of SNPs,and it was selected to develop the liquid chip,named“Melon2K”.Using Melon2K,more than 1500 SNPs were detected across 17 samples of five melon cultivars,and the phylogenetic relationships were clearly constructed.Within the same cultivar,genetic differences were also assessed between different samples.We evaluated the performance of Melon2K in genetic background selection during the breeding process,obtaining the introgression lines of interested trait with more than 97%genetic background of elite variety by only two rounds of backcrossing.These results suggest that Melon2K provides a cost-effective,efficient and reliable platform for genetic analysis and molecular breeding in melon.