tdTomato转基因小鼠的建系及其在细胞示踪方面的应用研究

目的构建稳定表达的tdTomato转基因小鼠并建系,观察其细胞及组织的荧光表达水平以及其干细胞共培养后的荧光表达水平。方法使用Gateway clone技术和DNA显微注射法构建含有tdTomato表达载体的受精卵,移植至假孕母鼠体内,待其自然生产。使用双向鉴定法鉴定并挑取饲养阳性小鼠并建系。另提取tdTomato阳性小鼠的神经干细胞分别与eGFP小鼠的骨髓间充质干细胞、原代神经干细胞共培养。结果成功构建了tdTomato转基因小鼠并建系,与野生型小鼠相比,tdTomato转基因小鼠生化指标和生长性状无明显差异,其组织切片及脑源神经干细胞均可观察到红色荧光。示踪实验表明注射部位可观察到明显的荧光成像,共培养实验可以清晰的观察到细胞分化后荧光的稳定表达。结论tdTomato转基因小鼠的组织和细胞能稳定表达红色荧光,可以利用荧光鼠的自发荧光特性,研究干细胞共培养后的分化方向。

大豆慢生根瘤菌3种标记载体构建与应用

大豆与根瘤菌的共生固氮是农业生态系统中主要的氮来源之一,研究其互作机制意义重大,但是由于根瘤菌个体小,转化难,目前尚缺乏高效、稳定标记根瘤菌的方法,限制了其在互利共生方面的研究。为开发用于大豆与慢生根瘤菌互作研究的根瘤菌标记方法,本研究通过改造原始载体pMG103,构建高效表达tdTomato、GUS、LUC的标记载体,以高效固氮的慢生根瘤菌株系Bradyrhizobium elkanii BXYD3为试验菌株,采用电击转化法进行标记。利用显微镜、GUS染液、化学成像仪观察标记的B.elkanii BXYD3根瘤菌在大豆不同时期不同部位的定殖情况。结果表明:成功获得了tdTomato、GUS及LUC标记的慢生根瘤菌转化菌株,携带不同标记的慢生根瘤菌株B.elkanii BXYD3能在大豆根表及根瘤内稳定定殖,并且可满足不同试验需求。本研究建立了较为稳定的表达多种标记蛋白的载体,且能较好地应用于慢生根瘤菌株系中,为直观研究大豆与慢生根瘤菌的互作提供有效的方法参考。

基于Cre-LoxP系统的B细胞特异性荧光报告基因小鼠模型的构建及鉴定

目的应用Cre^(-)LoxP重组酶系统构建B细胞特异性表达tdTomato蛋白的荧光报告基因小鼠。方法在Gt(ROSA)26Sor(Rosa26)位点插入1个由CAG启动子驱动的报告基团,其LoxP侧翼设计有STOP盒,可阻止tdTomato荧光蛋白表达,经与CD19-Cre工具小鼠交配繁殖获得tdTomato^(CD19-Cre)小鼠,Cre重组酶特异性识别LoxP序列,删除STOP盒,从而使B细胞特异性表达tdTomato荧光蛋白。利用PCR进行基因型鉴定。通过流式细胞术和脑膜免疫荧光分别检测野生型对照组小鼠和tdTomato^(CD19-Cre)荧光报告基因小鼠脾和脑膜B细胞中tdTomato红色荧光蛋白表达。结果基因型为tdTomato^(F/-)CD19-Cre^(+)或tdTomatoF/FCD19-Cre^(+)的小鼠为B细胞特异性表达tdTomato天然红色荧光蛋白的荧光报告基因小鼠。而对照组小鼠基因型为tdTomato^(F/-)CD19-Cre^(-)或tdTomatoF/FCD19-Cre^(-)。流式细胞术测定结果表明,与野生型对照组小鼠相比,tdTomato^(CD19-Cre)荧光报告基因小鼠脾中表达tdTomato荧光蛋白的B细胞百分比均显著增加(P<0.01);在非B细胞群中仅检测到少量的tdTomato+细胞。且在滤泡型B细胞、边缘区B细胞、T1 B细胞、T2 B细胞和成熟B细胞等B细胞亚群细胞表面tdTomato荧光蛋白均能稳定表达(P<0.01),百分比分别为(88±8)%,(80±9)%,(86±9)%,(92±6)%和(89±7)%。通过与CD45共定位,在tdTomato^(CD19-Cre)荧光报告基因小鼠脑膜中也检测到tdTomato红色荧光蛋白表达。结论成功构建B细胞特异性表达tdTomato荧光蛋白的荧光报告基因小鼠模型,且tdTomato荧光蛋白可在外周免疫器官和中枢神经系统稳定表达。

大鼠品系PGR-iCre构建

采用CRISPR/Cas9基因编辑技术首次制备用于子宫基因敲除的PGR-iCre大鼠。PGR-iCre大鼠与含有Flox报告基因Tdtomato大鼠(Tdtomatof/f)杂交得到PGRCre+/-- Tdtomatof/+大鼠。利用real-time PCR、免疫组化、荧光检测等技术检测Tdtomato基因在PGRCre+/-- Tdtomatof/+大鼠不同器官表达,间接检测PGR驱动的Cre重组酶组织特异性表达。结果表明,PGR驱动Cre重组酶在大鼠子宫、卵巢、输卵管、乳腺、下丘脑、垂体、脾脏、肾脏、肺等器官不同程度表达;未检测到Cre重组酶在心脏、肝脏、肌肉中表达。综上,PGR-iCre大鼠可作为子宫基因敲除工具鼠研究大鼠子宫表达基因的相关功能。

多巴胺D1受体在小鼠大脑皮层的空间分布研究

目的:利用多巴胺受体1(D1Rs)荧光转基因小鼠系统探讨D1Rs在小鼠大脑皮层的空间分布特征和相对表达模式。方法:使用成年Drd1-tdTomato转基因小鼠,制备冠状全脑切片,采用DAPI衬染细胞核,在共聚焦显微镜下观察D1Rs的分布,使用Imaris软件荧光阈值点自动计数算法实现细胞计数。结果:D1Rs在大多数大脑皮层区域内都有表达,但总体比例较低,这些区域包括眶皮层、岛叶皮层、扣带皮层、视皮层、听觉皮层、运动皮层、躯体感觉皮层、外嗅皮层和梨状皮层等。同时我们发现D1Rs在大脑皮层中主要集中在浅层(1/2层)和深层(5/6层)。结论:不同大脑皮层区域D1Rs分布模式不同。

Cell fusion in the liver, revisited

There is wide agreement that cell fusion is a physiological process in cells in mammalian bone, muscle and placenta. In other organs, such as the cerebellum, cell fusion is controversial. The liver contains a considerable number of polyploid cells: They are commonly believed to originate by genome endoreplication, although the contribution of cell fusion to polyploidization has not been excluded. Here, we address the topic of cell fusion in the liver from a historical point of view. We discuss experimental evidence clearly supporting the hypothesis that cell fusion occurs in the liver, specifically when bone marrow cells were injected into mice and shown to rescue genetic hepatic degenerative defects. Those experiments-carried out in the latter half of the last century-were initially interpreted to show "transdifferentiation", but are now believed to demonstrate fusion between donor macrophages and host hepatocytes, raising the possibility that physiologically polyploid cells, such as hepatocytes, could originate, at least partially, through homotypic cell fusion. In support of the homotypic cell fusion hypothesis, we present new data generated using a chimera-based model, a much simpler model than those previously used. Cell fusion as a road to polyploidization in the liver has not been extensively investigated, and its contribution to a variety of conditions, such as viral infections, carcinogenesis and aging, remains unclear.

DEVELOPMENT OF NEEDLE-BASED MICROENDOSCOPY FOR FLUORESCENCE MOLECULAR IMAGING OF BREAST TUMOR MODELS

Fluorescence molecular imaging enables the visualization of basic molecular processes such as gene expression,enzyme activity,and disease-specific molecular interactions in vivo using targeted contrast agents,and therefore,is being developed for early detection and in situ characterization of breast cancers.Recent advances in developing near-infrared fluorescent imaging contrast agents have enabled the specific labeling of human breast cancer cells in mouse model systems.In synergy with contrast agent development,this paper describes a needle-based fluorescence molecular imaging device that has the strong potential to be translated into clinical breast biopsy procedures.This microendoscopy probe is based on a gradient-index(GRIN)lens interfaced with a laser scanning microscope.Specifications of the imaging performance,including the field-of-view,transverse resolution,and focus tracking characteristics were calibrated.Orthotopic MDA-MB-231 breast cancer xenografts stably expressing the tdTomato red fluorescent protein(RFP)were used to detect the tumor cells in this tumor model as a proof of principle study.With further development,this technology,in conjunction with the development of clinically applicable,injectable fluorescent molecular imaging agents,promises to perform fluorescence molecular imaging of breast cancers in vivo for breast biopsy guidance.