Transienttransfectioninto293Tcells
PurposeTransient transfection into 293T cells is a convenient way to overexpress and obtain both cellular and extracellular (secreted or membrane) proteins. 293 is a human renal epithelial cell line which is transformed by adenovirus E1A gene product. 293T is a derivative which also express SV40 large T antigen, allowing episomal replication of plasmids containing the SV40 origin and early promoter region. They (both......阅读全文
Transient-transfection-into-293T-cells
PurposeTransient transfection into 293T cells is a convenient way to overexpress and obtain both cellular and extracellular (secreted or membrane) pro
Transient-Transfection-of-Cos1-Cells
Transient Transfection of Cos-1 CellsNote: This protocol has been optimized for Cos-1 cells. Successful transfection of each cell type requires optimi
Transfection-of-Mammalian-Cells-Using-Lipofectamine
Materials: LipofectamineBasal Medium containing 10% fetal bovine serum, 1% glutamine, 1% aaBasal Medium containing 1% glutamineBasal Medium cont
DNA转染
DNA转染· Transfection of Mammalian Cells Using Lipofectamine (LTI)· Guide to Eukaryotic Transfections with Cationic Lipid Reagents (PDF)
Growth,-Maintenance-and-Transfection-of-Suspension-Adapted-293EBNA-cells
ProcedureI. INTRODUCTIONThe 293 EBNA cell line is established from primary embryonal human kidney cells transformed with sheared human adenovirus type
Transfection-with-PEI
实验概要Use PEI (Linear 25 kDa Reagent) to transfect in HEK293T cells.主要试剂PEI is polyethyleimine, a 25 kDa linear from Polysciences Inc. Make up solutio
Production-of-neuronpreferential-lentiviral-vectors
实验概要Adenoviral vectors widely used to transfer foreign genes into neuronal cells possess tropism for glial cells and are toxic to infected cells.
Enzyme-Kinetics-assay-of-the-WT
To assay 17 b-HSD activity in lysates, cells were harvested 48h after transfection using PBS Enzyme Free Cell Dissociation Solution ( specialty Media
用CRISPR/Cas9对CART细胞进行多重基因编辑(二)
细胞系 Cell linesThe following CD19-expressing immortalized cell lines were used: Raji (Burkitt’s lymphoma cell line, ATCC-CCL86),Daudi (B lymphoblast ce
Generating-stable-cell-lines-in-HEK293
Generating stable cell lines in HEK293Prior to transfection, it is recommended that you linearize your pcDNA gene construct. Linearizing will decrease
Generating-stable-cell-lines-in-HEK293
Generating stable cell lines in HEK293Prior to transfection, it is recommended that you linearize your pcDNA gene construct. Linearizing will decrease
LentiVirus-Protocol
Lenti-Virus Protocol张端午A. For packing virus in 6-well plate: (if in 12-well plate, reduce all to 1/2)1. Mix the following plasmids in a 1.5 ml eppendo
Retrovirus-Production
Material:Packaging Cells, e.g. Phoenix cells (an adenovirus Ad5-transformed human embryonic kidney cell line 293T, transfected with two MoMLV packagin
Hematopoietic-Stem-Cell-Targeting-with-Surface1
Hematopoietic Stem Cell Targeting with Surface-Engineered Lentiviral VectorsEls Verhoeyen and François-Loïc CossetAdapted from Gene Transfer: Delivery
慢病毒转染肝细胞方法
Lentivirus Transduction of Hematopoietic CellsMing-Jie Li and John J. RossiDivision of Molecular Biology, Beckman Research Institute of the City of Ho
293fectin™-Transfection
实验概要293fectin™ is a proprietary, cationic lipid-based formulation for transfection of DNA into eukaryotic cells. 293fectin™ is optimized for transfe
Coimmunoprecipitation-assays
co-IP assays can be performed between endogenous proteins or transiently or stably expressed exogenous - usually tagged - proteins. The advantage to u
CoIP
Protocol for Co-IP of different proteins with RFP-MeCP2Preperation of cells (for p100):• 1st day split 293T EBNA cells in DMEM (high glucose +
Angiotensin-Protein-Kinase-Assay
James Hardwick's angiotensin assay protocolThis specific procedure was developed to assay the activity of the Lck kinase expressed from a retrovir
James-Hardwicks-angiotensin-assay-protocol
This specific procedure was developed to assay the activity of the Lck kinase expressed from a retroviral vector in rat fibroblasts. You can obviousl
Transfection-of-siRNA-oligos-to-peritoneal-macrophages
Use DeliverX Transfection from PanomicsModified protocol belowStep 1: Make complexesNote: Do not scale up more than 3xThaw siRNA and DeliverX reagen
Reverse-Transfection-for-Gene-Function-Analysis
This guide describes a microarray-based system for the functional analysis in mammalian cells of many genes in parallel. Mammalian cells are cultured
293T细胞的培养
包装细胞293T细胞的培养一、293T细胞的冻存1. 随着传代的次数增加,293T细胞会出现生长状态下降,出现突变等。所以要在细胞购进时就进行大量冻存,以保证实验的稳定性和持续性。2. 在细胞对数生长期进行冻存,增加细胞复苏成活率。3. 倒去细胞上清液,加入D-Hank's液洗去残留的培养基
细胞转染(Cell-Transfection)技术综述
一、细胞转染途径转染大致可分为物理介导、化学介导和生物介导三类途径。电穿孔法、显微注射和基因枪属于物理介导技术;化学介导方法很多,如经典的磷酸钙共沉淀法、脂质体转染方法、和多种阳离子物质介导的技术;生物介导方法,有较为原始的原生质体转染,和现在比较多见的各种病毒介导的转染技术。1、物理介导(1)电穿
Transfecting-Plasmid-DNA-into-NIH3T3-Cells-Using-Lipofectamine™-LTX-Reagent
实验概要Lipofectamine™ LTX Reagent is a proprietary, animal-origin free formulation for the transfection of DNA into eukaryotic cells with low cytotoxic
Transfecting-Suspension-Cells
实验概要将转移基因整合到细胞染色体DNA上,形成稳定表达转移基因的细胞系。 实验原理 细胞转染技术是目前广泛应用于病毒基因结构与功能以及基因调控等的研究。细胞转染可分为短暂转染和稳定(或永久) 转染两种。在短暂转染中,被转染基因并不整合至细胞染色体中,因而不能随细胞分裂而传代。转入病毒基因的转
表皮细胞的转染实验技巧
表皮细胞广泛遍布于身体,正常的表皮细胞较难转染,尤其是使用基于脂质体技术的转染试剂。我们使用电转(Amaxa)方法转染正常人的结肠表皮细胞并得到了65%的GFP标记细胞。非常感谢SignaGen,现在我们使用GenJet Ver II可以成功转染正常人的结肠表皮细胞并且转染效率显著提高至75%。
Differentiate-ES-cells-into-glial-cells-and-neurons
Day -1: Pass ES cells at normal density on gelatinized plate to free the culture of contamination fibroblast cells.___________________Day 1: Trypsiniz
Culture-of-BEND-Cells-(Bovine-Endometrial-Cells)
Culture of BEND Cells (Bovine Endometrial Cells)Charles E. Krininger, III and Peter J. Hansen Dept. of Animal Sciences, University of FloridaThis prot
稳定转染的基本概念
一般来说(由细胞类型决定),形成稳定转染细胞的效率比瞬时转染(transient transfection)的效率低1到2个数量级。利用可选择的遗传标记物有利于从非转染细胞的中分离出稀少的稳定转染物。