注射性组织工程牙胚的构建及成牙能力研究

目的:探索采用大鼠牙胚细胞构建可注射组织工程牙齿的可行性及在体内肾被膜移植的成牙能力研究。方法:采用出生后4d SD仔鼠磨牙牙胚细胞,培养传代后将牙胚细胞与牛真皮基质蛋白溶液混合构建组织工程牙胚,利用注射器植入SD大鼠肾被膜下,2wk后取材,HE染色观察移植物中的组织成熟情况,Masson’s三色法观察组织工程牙胚的成牙能力。结果:组织工程牙胚移植后2wk可在肾被膜下形成乳白色矿化组织,HE染色上皮细胞和间充质细胞进行重组,形成典型的牙髓牙本质复合体样组织和釉质样结构,Masson’s三色法可见绿色矿化基质形成并包绕牙乳头样组织。结论:牙胚细胞仍保留了牙齿发育的位置信息,采用牛真皮基质蛋白溶液作为组织工程支架有助于牙胚细胞相互作用并重新排列,构建的组织工程牙胚具有进一步成熟、矿化并形成牙齿的潜能。     

The formation of improved tetraploid population of red crucian carp × common carp hybrids by androgenesis

Bisexual fertile diploid androgenetic individuals (A0) (2n=100) were formed by androgenesis. In this way, the diploid spermatozoa from male allotetraploid hybrids (AT) (4n=200) of red crucian carp (Carassius auratus red var.) (♀) × common carp (Cyprinus carpio L.) (♂) were used to fertilize the UV-treated hap- loid eggs of goldfish (Carassius auratus), and living androgenetic diploid fish were developed. The A0 became sexually mature at the age of 2 years, and they fertilized with each other to form their offspring (A1). In this study, we observed the chromosomal number, gonadal structure and appearance of A1 fish. The results are as follows: (1) In A1, there were 85% tetraploids (A1-4n), 10% triploids (A1-3n) and 5% diploids (A1-2n), suggesting that diploid A0 could produce diploid gametes. It was concluded that the formation of diploid gametes generated from diploid A0 was probably related to the mechanism of pre-meiotic endoreduplication. (2) Among A1, only A1-4n possessed normal ovaries and testes. The mature males of A1-4n produced white semen. Under the electron microscope, the head of diploid sperm generated by A1-4n was bigger than that of haploid sperm generated by red crucian carp. In the testes of the A1-4n, there were many mature normal spermatozoa with a head bearing plasma mem- brane and a tail having the typical structure of "9 2" microtubules. Between the head and the tail, there were some mitochondria. The ovaries of A1-4n developed well and mainly contained II, III and IV-stage oocytes. The IV-stage oocytes were surrounded by inner and outer follicular cells. The micropyle was observed on the oolemma of follicular cells. There were abundant yolks and plenty of endoplasmic reticulum in the cytoplasm of IV-stage oocytes. Because A1-2n and A1-3n were distant crossing diploid hybrids and triploid hybrids respectively, they possessed abnormal gonads, and no mature semen and eggs were observed. (3) Compared with allotetraploids, the A1-4n fish not only had advantages such as fast growth rate and strong resistibility but also showed some new good performances such as high ratio of body width to body length, smaller heads and shorter tails. These results indicated that an- drogenesis could produce bisexual fertile tetraploids and improve the shape of allotetraploid hybrids as well, which will be of great significance in both the cell genetics research and fish breeding.     

核酸试纸条检测方法研究进展*

凝胶电泳、实时荧光PCR等常规核酸检测方法存在操作繁琐、设备昂贵、反应时间长等局限性。随着核酸检测市场规模的大幅提升,常规检测方法已无法满足临床诊断、检验检疫的需求。核酸试纸条(nucleic acid detection strip,NADS)是一种新兴的核酸检测方法,具有灵敏度高、操作便捷、结果可视化、成本低且耗时短等优势,在基础研究与临床诊断等领域受到广泛关注。综述近年来NADS的检测方法及研究进展,系统总结该技术的原理、应用及临床潜在转化价值,以期为NADS的进一步开发、利用提供借鉴。     

VdToxD1和VdToxD3调控大丽轮枝菌微菌核的萌发

大丽轮枝菌Verticillium dahliae是一种土传性植物病原真菌,可侵染660多种植物,引发黄萎病。微菌核是大丽轮枝菌在侵染后期形成的特殊休眠结构,可在土壤中存活14年,是黄萎病的主要初侵染来源。本研究在前期大丽轮枝菌萌发与休眠微菌核转录组分析的基础上,选择微菌核休眠状态高表达的VdToxD1和VdToxD3基因进行功能研究。结果发现,VdToxD1和VdToxD3敲除突变体菌株的微菌核萌发率分别为87.3%和86.0%,显著高于野生型菌株的64.0%;负调控微菌核萌发的转录因子VdCrz1与VdToxD1上游的-937 bp到-349 bp中的特定基序结合,与VdToxD3上游的-752 bp到-496 bp中的特定基序结合,结合位点均位于2个基因的启动子区。     

二代益生菌嗜黏蛋白阿克曼菌与慢性疾病的研究进展

随着人们对肠道菌群研究的深入,越来越多的证据表明肠道菌群失调与许多慢性疾病的发生和进展密切相关。目前,采用益生菌治疗疾病已成为国际热点,而嗜黏蛋白阿克曼菌(Akkermansia muciniphila,A. muciniphila)作为人类肠道黏液层中的常见定植菌,逐渐被认为是二代益生菌中有前途的候选者。本文综述了A. muciniphila对慢性疾病的改善作用及其可能机制,从而为疾病治疗提供新思路。     

GSK3β/eEF2K信号通路对小鼠肺纤维化过程的影响*

目的: 探讨糖原合成酶激酶-3(GSK3β)/真核延伸因子激酶2(eEF2K)信号通路对肺纤维化进程的影响,为临床治疗肺纤维化寻找新的思路。方法: 采用一次性气管注射法构建C57BL/6雄性小鼠博莱霉素肺纤维化模型,造模14 d后将动物分成模型组、阴性抑制组与抑制组(n=5),另设空白组不作处理。抑制组使用腹腔注射TDZD-8(4 mg/kg),阴性抑制组腹腔注射二甲基亚砜(DMSO)溶液,28 d后处死采集指标。采用苏木精-伊红染色法检测小鼠肺脏病变情况;试剂盒水解法检测肺组织中羟脯氨酸(Hyp)的含量;采用Western blot法检测肺脏中GSK3β、磷酸化GSK3β(p-GSK3β)、eEF2K、p-eEF2K(Ser70)、p-eEF2K(Ser392)、p-eEF2K(Ser470)、基质金属蛋白酶-2前体蛋白(pro-MMP-2)、基质金属蛋白酶-2(MMP-2)蛋白表达水平,使用免疫组织化学法检测肺脏中MMP-2、胶原蛋白I(Col I)、胶原蛋白Ⅲ(Col Ⅲ)、α-平滑肌蛋白(α-SMA)的表达。结果: 与空白组相比,模型组中GSK3β、p-GSK3β、p-eEF2K(Ser70)、p-eEF2K(Ser392)、p-eEF2K(Ser470)、pro-MMP-2、MMP-2、Col I、Col Ⅲ、α-SMA蛋白表达水平升高,eEF2K蛋白表达水平降低(P＜0.05);与模型组相比,抑制组GSK3β、p-GSK3β、p-eEF2K(Ser70)、p-eEF2K(Ser392)、p-eEF2K(Ser470)、pro-MMP-2、MMP-2、Col I、Col Ⅲ、α-SMA蛋白表达降低,eEF2K蛋白表达升高(P＜ 0.05)。结论: GSK3β能通过Ser70、Ser392、Ser470这3个位点磷酸化激活eEF2K,增加纤维化指标含量,促进肺纤维化形成,加重肺组织病变。     

土壤呼吸对降雨变化和氮沉降交互作用响应的研究进展

土壤呼吸作为陆地生态系统碳循环的关键过程,对大气CO₂浓度变化有直接影响。研究其如何响应降雨变化、氮沉降增加等全球变化因子,成为近年全球变化领域的热点与难点。与土壤呼吸响应降雨变化或氮沉降增加单个因子相比,研究土壤呼吸对这两个因子交互作用的响应更接近真实的自然环境,可更准确地预估未来土壤碳排放的变化趋势。目前,相关研究涉及全球不同的陆地生态系统,从土壤、微生物和植物层面对其响应机理进行揭示。本文从土壤呼吸及其组分、相关的土壤性质、微生物及植物因素方面,较全面地梳理了不同陆地生态系统土壤呼吸响应降雨变化和氮沉降增加交互作用的研究进展,指出了现有研究中的不足及今后需加强的研究方向,以期为进一步揭示土壤呼吸对降雨变化和氮沉降增加交互作用的响应规律及机制提供参考。     

心肌缺血再灌注手术改变炎症相关肠道菌群

目的探讨心肌缺血再灌注损伤对大鼠肠道菌群结构特征的影响。方法18只雄性Sprague Dawley大鼠随机分为假手术组(n=7)和模型组(n=11),分别对大鼠冠状动脉左前降支进行结扎和再灌注。再灌注60 min后,通过TTC染色检测总梗死面积,H&E染色和免疫组织化学观察炎症细胞浸润情况、16S rRNA高通量测序分析心肌缺血前和再灌注后粪便中微生物的结构组成变化。结果与假手术组相比,模型组心肌梗死面积增加,心肌中炎症细胞浸润以及CD68阳性巨噬细胞明显增多,变形菌门(Proteobacteria)的相对丰度增加,厚壁菌门(Firmicutes)的相对丰度降低。结论心肌缺血再灌注损伤改变了肠道菌群的分布,这可能与促进了受损心脏的炎症细胞浸润有关。     

植物子平台及中国数字植物标本馆(CVH)运维: 做法和经验

该文系统介绍了植物子平台所采取的以数字标本质量为导向的数字化技术规范和管理策略,以及CVH网站数据共享规则, 并指出存在的问题及今后努力方向。