[3H]CholineLabelingandTNFTreatmentofHL60Cells
1) Grow cells to a density of 5-8 X 105 cells/ml in RPMI 1640 containing serum.2) Pellet cells and wash 1 time with room temperature PBS.3) Resuspend final pellet in an appropriate volume of prewarmed serum free media and supplement with ITS (4 ml/L should yield 5 mg/L insulin and 5 mg/L transferrin).--> "Appropriate" = bring cells to a final concentration of 2 X 105 cells/ml.4) Add (0.5 µl/ml media) [3H......阅读全文
[3H]-Choline-Labeling-and-TNF-Treatment-of-HL60-Cells
1) Grow cells to a density of 5-8 X 105 cells/ml in RPMI 1640 containing serum.2) Pellet cells and wash 1 time with room temperature PBS.3) Resuspend
Sphingomyelin-Quantitation-Postcholine-Labeling-of-HL60-Cells
Lipid Extraction1) Following the appropriate time of treatment, transfer 4.5 ml into each of two duplicate glass pyrex tubes and maintain on ice.2) Sp
Immunofluorescence-Labeling-of-Cells
实验概要Antibodies are an important tool for demonstrating both the presence and the subcellular localization of an antigen. Cell staining is a very ver
RNAse-A-Treatment-of-Mouse-Cells
IntroductionRNAse A treatment of permeabilized cells followed by immunostaining is a method which allows to show if the localization of a protein into
Metabolic-Labeling-of-Cells-with-35S
1) Transfer to a 24 wells plate the desired colonies.2) Once the cells are attached (at least 8 hours after tripsinizing them) add ~1 ml ofDME (met-,
CIP-Treatment
set up the following reaction:CIP RxnH2O7.8 ml10x cip rxn buffer2.0 mlDNA(e.g; 3 kb vector; 0.2 mg/ml; 2 mg total)10.0 ml(1 u/ml) CIP0.2 mltotal20.0 m
Labeling-Tubulin-and-Quantifying-Labeling-Stoichiometry
Labeling Tubulin and Quantifying Labeling StoichiometryThis is a general procedure for coupling moieties with reactive succinimidyl esters to tubulin.
Labeling-Tubulin-and-Quantifying-Labeling-Stoichiometry2
II. Labeling ProtocolThe procedure described below can be scaled down if desired. It is essential to perform all steps involving caged dyes under a sa
TUNEL-labeling
In Situ Cell Death (Apoptosis) Detection by TUNEL labelingby Boehringer Mannheim (Catalog No. 1684809), modified by Josiah N. Wilcox andJosé C. Rodrig
Biosynthetic-labeling
How long should cells be labeled? The ideal length of time to label cells depends on the protein of interest and the label that you are using. If you
MITOMYCIN-C-TREATMENT-OF-PMEFs
Cultures to be treated should be sub confluent ie actively growing.1. Add 1/20 volume Mitomycin C (200 ug/ml 10 ug/ml), to culture and incubate at 37
CMFDA-Labeling-of-Platelet
OUTLINECMFDA (5-chloromethylfluorescein diacetate) is a lipophilic tracer that has an enormous advantage over ordinary tracers (e.g. FITC) because it
Arachidonic-Acid-Labeling
1) Grow cells to a density of 5-8 X 105 cells/ml in RPMI 1640 containing serum.2) Pellet cells and wash 1 time with room temperature PBS.3) Resuspend
BrdU-Labeling-Protocol
实验概要The thymidine analog, 5-bromo-2-deoxyuridine (BrdU),is a common reagent used for cell proliferation assays and for the detection of apoptotic
Detection-by-TUNEL-labeling
In Situ Cell Death (Apoptosis) Detection by TUNEL labelingby Boehringer Mannheim (Catalog No. 1684809), modified by Josiah N. Wilcox,José C. Rodriguez
Formaldehyde-Treatment-of-Tissue-Culture-Hoods
You will need:-12g Potassium Permanganate 6g Crushed paraformaldehyde1) Set the hood so that it can vent outside.2) Mix the two chemicals above togeth
流式细胞仪技术专辑
Flow Cytometry Analysis (Springer Lab, Harvard University) Flow cytometry employs instrumentation that scans single cells flowing past excitation sour
DNA-labeling-by-nick-translation
DNA labeling by nick translationreagents: DNA for labeling (concentration c > 150 ng/µl) modified nucleotides: Biotin-16-dUTP, Digoxigenin-11-dUTP, co
Radioactive-DNA-Fragmentation-Assay
DESCRIPTION of the method:The DNA Fragmentation Assay allows to determine the amount of DNA that is degraded upon treatment of cells with certain agen
RNase-and-DEPC-Treatment:-Fact-or-Laboratory-Myth
Researchers are usually trained in RNA isolation and analysis methods by one another or by technical manuals. Experimental procedures are often not qu
DNAse-posttreatment-for-nuclear-antigens
Rationale: The use of DNAse to improve nuclear antigen staining has been published long before the AR era 1, 2.DNAse treatment is currently suggested
用CRISPR/Cas9对CART细胞进行多重基因编辑(三)
流式细胞术 Flow cytometry CytoFLEX (Beckman Coulter Inc) was used to perform fluorescent expression analysis. Cells were harvested on the following day
流式细胞仪技术专辑
最方便的实验干货查询工具微信扫码进入「丁香实验」小程序编辑: 呜咽分享到: Flow Cytometry Analysis (Springer Lab, Harvard University)Flow cytometry employs instrumentation that scan
CD40L-Signaling-Pathway
The CD40 receptor was first associated with expression in B cells and the role it plays through its ligand CD40L (CD154) in moderating T cell activati
Basic-Method-for-Indirect-Immunofluorescence-Labeling
Basic Method for Indirect Immunofluorescence LabelingBackgroundThis is the method for indirect immunofluorescence labeling; that is, the antibodies do
Multicolour-3DFISH-in-vertebrate-cells2
Small DNA-probes from cosmids or plasmids clonesThese kind of probes, especially plasmids, have become out of fashion for 3D-FISH due to their delicat
The-41BBdependent-immune-response
The activation of T cells requires a co-stimulatory signal with T cell receptor activation, provided in many cases by activation of CD28 in resting T
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
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
ThiolReactive-Probe-Labeling-Protocol
实验概要Invitrogen offers several fluorescent and biotinylated phalloidin and phallacidin derivatives for labeling F-actin. These phallotoxins, isolated