ASENSITIVEMETHODFORDETECTIONOFAPOPTOSISBYSINGLELASERFLOWCYTOMETRY
MATERIALS:1. 1 X PBS (PBSAz, 1 X PBS, e.g., Irvine Scientific, CA, containing 2% newborn calf serum and 0.1% sodium azide)2. 7-Amino-actinomycin D (7-AAD, e.g., Calbiochem, CA)3. Human AB serum, heat-inactivated (HAB, e.g., Irvine Scientific, CA)4. Refrigerated centrifugePreparation of 7-AAD stock solutionDissolve 7-AAD powder (1mg) first in 50 microliters of absolute methanol, then add 950 microliters of 1 X PBS. Fi......閱讀全文
ASENSITIVE-METHOD-FOR-DETECTION-OF-APOPTOSIS-BY-SINGLE-LASER-FLOW-CYTOMETRY
MATERIALS:1. 1 X PBS (PBSAz, 1 X PBS, e.g., Irvine Scientific, CA, containing 2% newborn calf serum and 0.1% sodium azide)2. 7-Amino-actinomycin D (7-
Detection-Of-Cell-Viability-And/Or-Apoptosis-By-Flow-Cytometry-(FACS)
Viable?cells are cells that when allowed to continue beyond the timepoint of examination will stay alive. Besides live and healthy cells, cells in ear
Detection-of-Intracellular-Antigens-by-Flow-Cytometry
實驗概要Fix and Perm ?reagents are designed for use with all commercially available flow ?cytometers. Alignment and compensation should be performed accor
Apoptosis:-A-Laboratory-Manual-of-Experimental-Methods-Andrea-Cossarizza
THE CELL?1.?Morphological aspects of apoptosis?Walter Malorni, Stefano Fais & Carla Fiorentini?2.?Cell cycle?Miriam Capri & Daniela BarbieriTHE NUCLEU
specific-immunodetection-of-cyclins-using-488/630-dual-laser-flow-cytometry
Phenotype-specific immunodetection of cyclins using?488/630 nm dual laser flow cytometryWilliam Telford?Hospital for Special SurgeryThis protocol is f
流式細胞儀技術專輯
Flow Cytometry Analysis?(Springer Lab, Harvard University)?Flow cytometry employs instrumentation that scans single cells flowing past excitation sour
流式細胞儀技術專輯
?最方便的實驗干貨查詢工具微信掃碼進入「丁香實驗」小程序編輯:?嗚咽分享到:??????Flow Cytometry Analysis?(Springer Lab, Harvard University)Flow cytometry employs instrumentation that scan
Alexa-Fluor?-488-Annexin-V/Dead-Cell-Apoptosis-Kit
實驗概要Apoptosis is a ?carefully regulated process of cell death that occurs as a normal part ?of development. Inappropriately regulated apoptosis is imp
Simultaneous-analysis-of-DNA-content
Simultaneous analysis of DNA content and surface immunophenotype using gentle ethanol fixation techniques.??William Telford. Louis E. King and Pamela
An-Integrative-Procedure-for-Apoptosis-Identification-and-Measurement2
TroubleshootingCritical Steps(1) Don’t trypsinize cells for too long when collecting them.(2) Rotation speed should be no more than 1500 rpm during ce
Flow-Cytometry-Analysis
PurposeFlow cytometry employs instrumentation that scans single cells flowing past excitation sources in a liquid medium. The technology can provide r
JC1分析線粒體膜電位的方法3
3.6 Key references1. Kroemer G., Zamzani N., Susin S.A. Mitochondrial control of apoptosis.?Immunol. Today,?18: 44-51, 1997.2. Susin S.A., Zamzami N.,
FACS-Procedures-for-Apoptosis-Detection
Materials:Hoechst?33258?(Sigma B-2883).stock: 10 mg/ml in dH20 (40)working dilution: 500μg/ml (50μl stock + 950μl PBS).7-Amino-actinomycin (Sigma A-94
A-rapid-and-highly-sensitive-method-for-somatic-mutation-profiling
AbstractTumor genotyping can provide a useful guide to drive clinical trials, inform treatment options, and predict patient outcomes1. This is due, in
Yeast-Cell-Cycle-by-Flow-Cytometry
ReagentsCold absolute ethanol.0.5 M Na citrate stock (filtered), 50mM diluted stock.10 mg/ml RNase A (Boil 10 mins, cool, filter and store at -20°C).4
Intracellular-Immunofluorescent-Staining-for-Flow-Cytometry
IntroductionA modification of the basic immunofluorescent staining and?flow cytometric analysis protocol?can be used for the simultaneous analysis of
細胞周期的流式細胞伩檢測實驗方法(PI,Brdu)2
B.3. COMMENTARY?B.3.1 Background information?The critical steps in the methodology are cell fixation, permeabilization and the concentrations of anti-
Apoptosis-Induction
IntroductionWhen studying induction of apoptosis via a cell surface molecule, it is important to first ascertain surface expression of the molecule of
Combined-Flow-Cytometric-Measurement-of-Two-CellSurface-Antigens
INTRODUCTIONFlow cytometry is frequently used to assess nucleic acid content?in individual cells. Based on DNA content alone, however, cells?in the qu
A-rapid,-quantitative-and-inexpensive-method-for-detecting-apoptosis2
Figure?1.Determination of apoptosis in transiently transfected murine [beta] tumor cells. (A) The number of apoptotic [beta]HC 13T tumor cells (% apop
Flow-Cytometry-of-Fibroblast-Nuclei-for-DNA-content
MaterialsP.I. Solution:?4 mM Na3Citrate (0.118 g/100 mL)30 U/mL RNAseI (43 mg/100 mL)0.1% Triton-X100 (0.1mL/100 mL)50 μg/mL propidium iodide (5 mg/10
A-rapid,-quantitative-and-inexpensive-method-for-detecting-apoptosis
ASTRACTWe describe a rapid and quantitative flow cytometric method for determining the apoptotic or anti-apoptotic potential of a gene in various cell
Intracellular-Immunofluorescent-Staining-for-Flow-Cytometry2
Table 2: Human Cytokines: Intracellular Staining Quick GuideHuman Cytokines: Intracellular Staining Quick GuideHuman CytokineCell SourceActivationIncu
Application-Note:-Qdot?-Nanocrystal-Conjugates-in-Flow-Cytometry
實驗概要Researchers today ?are trying to maximize the information that they get out of flow ?cytometry experiments by looking at more parameters in a sing
流式細胞儀(Flow-Cytometry)
1 流式細胞儀的概念及其發展歷史1.1 流式細胞儀的基本概念 流式細胞儀(flow cytonletry,FCM)是對高速直線流動的細胞或生物微粒進行快速定量測定和分析的儀器,主要包括樣品的液流技術、細胞的計數和分選技術,計算機對數據的采集和分析技術等。流式細胞儀以流式細胞術為理論基礎,是流體力學、
流式細胞術(Flow-Cytometry,-FCM)
流式細胞術(Flow Cytometry, FCM)是一種在功能水平上對單細胞或其他生物粒子進行定量分析和分選的檢測手段,它可以高速分析上萬個細胞,并能同時從一個細胞中測得多個參數,與傳統的熒光鏡檢查相比,具有速度快、精度高、準確性好等優點,成為當代最先進的細胞定量分析技術。流式細胞儀(Flow C
流式細胞儀(Flow-Cytometry)
1?流式細胞儀的概念及其發展歷史1.1 流式細胞儀的基本概念 流式細胞儀(flow cytonletry,FCM)是對高速直線流動的細胞或生物微粒進行快速定量測定和分析的儀器,主要包括樣品的液流技術、細胞的計數和分選技術,計算機對數據的采集和分析技術等。流式細胞儀以流式細胞術為理論基礎,是流體力學、
In-Situ-Cell-Death-(Apoptosis)-Detection-by-TUNEL-labeling
Protocol for Frozen Sections:Warm 150ml 4% Paraformaldehyde/1x PBS to RT. Fix slides in it, 20 min., RT.1x PBS rinse, 2 times.1x PBS, 30 min., RT. Beg
Detection-of-MicroRNA-Heterogeneity-in-Single-Cells-Using-an-Automated
Introduction ?MicroRNA ?(miRNAs) are short (18–24 nucleotides), non-coding RNAs that regulate ?gene expression by both disrupting messenger RNA (mRNA
Combined-Flow-Cytometric-Measurement-of-Two-CellSurface-Antigens2
DNA and RNA Staining6. Stain cells with 7-AAD:?i. Resuspend the cells from Step?5 in 0.5 mL of NASS containing?10 μg/mL of 7-AAD. Incubatefor 20 min a