建筑施工便拆式高周转回顶支撑体系设计与工程应用实践

针对现代建筑施工中回顶支撑体系存在的拆卸不便、周转率低及成本高等问题,创新性设计了一种便拆式高周转回顶支撑体系,并深入探讨了其设计思路、结构特点、优势以及在实际工程中的应用效果。通过模块化设计、选用轻质高强材料以及优化连接方式,该体系实现了快速安装、便捷拆卸和高周转率,显著提升了施工效率并降低了成本。同时,该体系还注重环保与可持续性,符合现代建筑施工的发展趋势。在佛山凤桐花园项目一期的工程应用实践中,便拆式高周转回顶支撑体系展现了其在施工进度、质量、安全性和经济效益方面的卓越表现。研究结论表明,该体系不仅能够有效解决传统支撑体系的痛点问题,还具有较高的推广应用价值。

辐射制冷技术浅圆仓控温试验研究

将辐射制冷材料粘贴或涂刷于浅圆仓仓顶和外壁,试验表明:试验仓比对照仓仓顶外表面平均温度低4.3℃,最高值低26.1℃;平均仓温低2.8℃,最高值低5.6℃;平均粮面温度低2.4℃,最高值低4.7℃。试验表明,辐射制冷材料应用于浅圆仓具有显著的降温效果,新型辐射制冷技术产业化的突破为粮食仓储行业实现更高质量的仓储环境提供了新材料,为实现浅圆仓的准低温储粮提供了新的参考方法。

辐射制冷材料平房仓控温试验研究

通过在平房仓仓顶铺设辐射制冷卷材,探究辐射制冷材料在平房仓实仓应用的控温效果.研究表明,粮温上升阶段,试验仓粮温上升速率仅为对照仓的1/4;粮温下降阶段,试验仓粮温下降速率却是对照仓的1.25倍;持续高温天气条件下,仓房外顶温度、架空层温度、仓温和上层粮温(局部)最高降幅分别为27.1℃、20.6℃、8.8℃和3.1℃.辐射制冷材料为平房仓的节能控温提供新的参考途径.

CLN1型神经元蜡样脂褐质沉积症伴遗传性高铁蛋白血症-白内障综合征1例患儿的分析

目的分析1例神经元蜡样脂褐质沉积症1型(CLN1)合并遗传性高铁蛋白血症-白内障综合征(HHCS)患儿的临床及遗传学特征。方法以2020年11月郑州大学第一附属医院收治的1例患儿作为研究对象。收集患儿的临床资料,对其进行基因检测,并结合文献回顾分析其临床和遗传变异的特点,为早期识别提供思路。结果患儿男,3岁,以视力损害、进行性认知和运动功能倒退、癫痫发作为主要表现。磁共振成像提示双侧大脑半球脑沟加深、髓鞘发育明显落后。棕榈酰蛋白硫酯酶活力偏低(8.4 nmol/g/min,正常参考值:132.2~301.4 nmol/g/min),血清铁蛋白升高(2417.70 ng/mL,正常参考值:30~400 ng/mL)。眼底成像示视网膜色素变性。全外显子测序发现患儿PPT1基因存在c.280A>C及c.124-124+3delG复杂杂合突变,分别遗传自父亲和母亲,二者既往均未见报道。此外,其FTL基因存在c.-160A>G杂合变异,遗传自父亲。结合患儿的临床表型和遗传变异,诊断其为CLN1和HHCS。结论PPT1基因的c.280A>C和c.124-124+3delG复合杂合变异及FTL基因的c.-160A>C变异可能是患儿的遗传学病因。临床对于视力损害进展较快的CLN1患儿,应进一步完善眼科检查并详细询问家族史,对高度怀疑合并HHCS的患儿应尽早通过基因检测确诊。

Generation of VP5 deficient mutant of infectious bursal disease virus strain HZ2

Infectious bursal disease virus (IBDV) is a bi-segmented, dsRNA virus of the Birnaviridae family. The nonstructural protein VP5 has been re- ported to be associated with virus-induced cell apoptosis and pathogenicity, but its role in viral rep- lication has not been unequivocally identified. Based on a PCR introduced mutagenesis strategy, the 33 bp of 96―129 bp located between ORF A1and ORF A2 of genomic segment A of IBDV strain HZ2 were de- leted, and an Nhe I (GcTaGc) site was inserted at 96―102 bp simultaneously. The mutated segment A was ligated into pCI, resulting in pCI-ANhe3. A chi- meric and deficient IBDV strain, named strain ANhe3, was recovered from chicken embryo fibroblast (CEF) cells by co-transfection with pCI-ANhe3 and pCI-mB, derived from the genomic segment B strain HZ2. The indirect fluorescent assay identified that strain ANhe3 could replicate on CEF cells without expression of VP5. Further examination showed that the patho- genesis of strain ANhe3 replicating on SPF chicken embryos was attenuated compared to strain HZ2. This paper provides a new rapid rescue strategy for gene-deleted virus. This strategy lays a basis for gene-deleted vaccine of IBDV.