MeasurementofGreenFluorescentProteinExpression
ReagentsCells to be studied expressing green fluorescent protein (GFP). Note that the same cell type without GFP is needed as control.Hoechst 33342 stock solution (1mg/ml) (see recipe)12 X 75 mm culture tubesVortex mixerWaterbath at 37oCMethod1. Count cells.2. Place approximately 106 cells into a 12 x 15 mm test tube and spin them down by centrifugation for 5 min at 300 x g.3. Remove supernatant by aspirat......閱讀全文
Measurement-of-Green-Fluorescent-Protein-Expression
?ReagentsCells to be studied expressing green fluorescent protein (GFP). Note that the same cell type without GFP is needed as control.Hoechst 33342 s
Measurement-of-GFP-Expression-and-DNA-Content-in-Permeabilized-Cells
ReagentsCells to be studied expressing green fluorescent protein (GFP). Note that the same cell type without GFP is needed as a control.1 X PBS2% Buff
Green-Fluorescent-Protein-as-an-Indicator-ofTransfection-in-Chicken-Embryos
Green fluorescent protein (GFP) is responsible for the bioluminescence of the Pacific Northwest jellyfish, Aequorea victoria. In A.victoria, the 27-kD
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
In-Vivo-Imaging-of-Far1
In Vivo Imaging of Far-red Fluorescent Proteins after DNA Electrotransfer to Muscle TissueDNA electrotransfer to muscle tissue yields long-term, high
Protein-Expression-and-Purification-Protocol
Step 1:?Transform?appropriate DNA plasmid into BL21(DE3)?E. coli?cells. These cells must be competent. (Protocol for how to make competent cells.)a) T
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
CELL-CYCLE-ANALYSIS
PROPIDIUM IODIDE: The most commonly used dye for DNA content/cell cycle analysis is PROPIDIUM IODIDE (PI). It can be used to stain whole cells or isol
細胞周期的流式細胞伩檢測實驗方法(PI,Brdu)1
ANALYSIS OF CELL CYCLE?Miriam Capri and Daniela Barbieri?Dept. Biomedical Sciences, Sect. General Pathology,Via Campi, 287, University of Modena, 4110
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
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
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
SDSPAGE檢測蛋白表達(protein-expression)
一、材料與儀器30%丙烯酰胺溶液;1.5mol/L Tris-HCl分離膠緩沖液,PH8.8;1.0mol/L Tris-HCl濃縮膠緩沖液,PH6.8;電泳緩沖液,PH8.3;10%SDS溶液;10%過硫酸銨溶液;樣品處理液;染色液;脫色液;電泳玻璃板,電泳電源架,電泳槽,電泳儀等;蛋白Mar
Vybrant?-DyeCycle?-Green-and-Orange-Stains
實驗概要Live ?cell studies of cellular DNA content and cell cycle distribution are ?useful to detect variations of growth patterns due to a variety of ?ph
In-Vivo-Imaging-of-Far3
To determine the minimum dose of Katushka plasmid needed to give detectable fluorescent intensity, we decreased the amount of pTurboFP635 to 0.5 and 1
Realtime-PCR
實驗概要The ?exponential amplification via reverse transcription polymerase chain ?reaction provides for a highly sensitive technique in which a very low
Vybrant?-DyeCycle?-Violet-Stain
實驗概要Live cell studies ?of cellular DNA content and cell cycle distribution are useful to detect ?variations of growth patterns due to a variety of phy
DAPI染DNA的原理及使用方法
DAPI ?即4',6-二脒基-2-苯基吲哚(4',6-diamidino-2-phenylindole),分子式為C16 H15 N5 ·2C3 H6 O3 ,分子量457.48。DAPI 是一種能夠與DNA強力結合的熒光染料。它結合到雙鏈DNA小溝的AT堿基對處,一個DAPI分子
DAPI染DNA的原理及使用方法
DAPI 即4',6-二脒基-2-苯基吲哚(4',6-diamidino-2-phenylindole),分子式為C16 H15 N5 ·2C3 H6 O3 ,分子量457.48。DAPI 是一種能夠與DNA強力結合的熒光染料。它結合到雙鏈DNA小溝的AT堿基對處,一個DAPI分子可
什么是gfp蛋白及其應用
綠色熒光蛋白GFP的研究進展及應用作者:吳沛橋~巴曉革~胡海~趙靜【摘要】 源于多管水母屬等海洋無脊椎動物的綠色熒光蛋白(GFP)~是一種極具應用潛力的標記物~有著極其廣泛的應用前景。我們就GFP的理化性質、熒光特性、改進和應用研究進行了綜述。【關鍵詞】 綠色熒光蛋白,GFP,,標記物,熒光特性,進
Dynamic-Monitoring-ofCellular-Remodeling-Induced-bythe-Transforming-Growth1
The plasticity of differentiated adult cells could have a great therapeutic potential, but at the same time, it is characteristic of progression of se
Fluorescent-Staining-of-Cells
1. Fluorescent phalloidin in methanol. Phallacidin does not work as well. Dilute 10 ul 330 nM stock into 500 ul PBS for each large coverslip.2. PB
蛋白質提取和純化
蛋白質提取和純化(主要內容如下)Protein Extraction?Protein PurificationProtein PrecipitationColumn PreparatioinQ & A Posted in the Method ForumProtein ExtractionWhole
Vybrant?-DyeCycle?-Ruby-stain
實驗概要Live cell studies ?of cellular DNA content and cell cycle distribution are useful to detect ?variations of growth patterns due to a variety of phy
PCR基因芯片上熒光PCR反應的研究(五)
3.討論 ?隨著近年基因芯片技術的發展,研究者逐漸認識到基于核酸雜交原理的傳統基因芯片缺陷與應用的局限性。隨著PCR技術的進展,特別是熒光定量PCR技術的出現PCR技術已成為生物醫學領域中應用最廣泛的技術。如果一種基因芯片能直接進行PCR反應,而且能夠同時擴增大批可能發生變異的基因顯然會有廣泛
DNA微序列技術
·?????????Protocols for Making Drosophila Arrays?(Stanford U.)Detailed protocol for making arrays including PCR Amplification of cDNAs for Printing,?
分光光度計知識
With the aid of spectroscopy, the quantitative analysis of nucleic acids and proteins has established itself as a routine method in many laboratories.
Quantification-made-easy
With the aid of spectroscopy, the quantitative analysis of nucleic acids and proteins has established itself as a routine method in many laboratories.
分光光度計的使用
With the aid of spectroscopy, the quantitative analysis of nucleic acids and proteins has established itself as a routine method in many laboratories.