InVivoImagingofFar1
In Vivo Imaging of Far-red Fluorescent Proteins after DNA Electrotransfer to Muscle TissueDNA electrotransfer to muscle tissue yields long-term, high levels of gene expression; showing great promise for future gene therapy. We want to characterize the novel far-red fluorescent protein Katushka as a marker for gene expression using time domain fluorescence in vivo imaging. Highly efficient transgenic expression was ob......閱讀全文
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
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
In-Vivo-Imaging-of-Far2
In vivo bio-imaging?? Mice were anesthetized and placed in a custom-made bed, which allowed stable and reproducible imaging of the legs. In vivo scann
In-Vivo-Luciferin-Imaging-Procedure
Mice are injected by an intraperitoneal route with a Luciferin solution (15 mg/mL or 30 mg/kg, in PBS, dose of 150 mg/kg) that is allowed to distribut
Live-imaging-with-Drosophila-tissue-culture-cells1
IntroductionLive imaging provides an important complementation to the "snapshot" view obtained in fixed tissue by immunofluorescence. It allows follow
Protein-detection-onto-PVDF-membranes
2-D PAGE and electroblotting onto PVDF membranes have become widely used techniques for the characterization of proteins. Recent improvements have all
通過細胞受體代謝生物素化進行圖像分析
Metabolic biotinylation of mammalian cell receptors for imagingBakhos A. Tannous , btannous@hms.harvard.edu, Massachusetts General Hospital and Harvar
Western-Blotting-Protocols
back to topProtocolStandard vs. Rapid Immunodetection ProceduresThere are two types of protocols for immunodetection: Standard and rapid.Standard vs.
條帶轉移(Band-Shift)
Or gel mobility shift assay, gel shift assay, gel retardation, electrophoretic mobility shift assay (EMSA)?EMSA Using Oligos?(Mike A. Dyer)Anneal two
體外熒光法檢測核內體早期動力學6
Critical step?Be careful to thaw PNS and cytosol slowly on ice to avoid unwanted protein degradation or breaking of organelles. This might require up
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
DNA-Immunoprecipitation-for-the-Determination-of-DNABinding-Specificity
Andrea J. Gossett?and?Jason D. Lieb1Department of Biology, University of North Carolina at Chapel Hill, Chapel Hill, NC 27599, USA1Corresponding autho
時域體內熒光成像技術應用于實驗性腦中風血腦...(六)
盡管根據本研究中的數據判斷是引人注意的并且可以推斷使用小的和大的MW示蹤劑的BBB替代半影成像生物標記物的空間分布不同。類似的磁共振成像分析的擴散灌注錯配模型,這些研究的缺點會阻礙確切的結論。與Nagaraja和他的同事的研究相比,本研究中使用Cy5.5和BSA-Cy5.5早分組的動物中,不平等交付
Live-Cell-Imaging-of-Yeast
Live Cell Imaging of YeastDaniel R. Rines, Dominik Thomann, Jonas F. Dorn, Paul Goodwin and Peter K. SorgerINTRODUCTIONThe development of cloning vect
Fluorescence-Procedures-fortheActin-andTubulin-Cytoskeleton-in-Fixed-Cells2
Formaldehyde FixationFix in 4% formaldehyde (16% stock EM grade) in CBS for 20 minutesRinse in TBSPermeabilize as for methanol fixationProcede as for
體外熒光法檢測核內體早期動力學
A fluorescence-based?in vitro?assay for investigating early endosome dynamicsSina V Barysch1,2, Reinhard Jahn1?& Silvio O Rizzoli2ABSTRACTEarly endoso
人工轉錄因子的部件——人類鋅指結構1
Human zinc fingers as building blocks in the construction of artificial transcription factorsKwang-Hee Bae1, 4, Young Do Kwon1, 2, 4, Hyun-Chul Shin1,
重組DNA的分離、克隆與測序實驗手冊8
B. Midiprep double-stranded DNA isolationA midi-prep double-stranded DNA isolation has been developed to generate a sufficient amount of template DNA
Fluorescence-Procedures-forthe-ActinandTubulin-Cytoskeleton-inFixed-Cells2
Actin CytoskeletonMethanol fixationFix in -20oC methanol for 1-2.5 minutesRinse in TBSPermeabilize in TBS-0.5% TX for 10 minutesRinse in TBS-0.1% TX (
體外熒光法檢測核內體早期動力學2
Full size image (70?KB)In vitro?incubation of a reaction mix that contains labeled endosomes, cytosol and an ATP-regenerating system at physiological
Immunocytochemistry...
實驗概要The ?green fluorescent protein (GFP) from the jellyfish Aequorea victoria is ?a versatile marker for monitoring physiological processes, visualizi
Purification-of-MBP-(maLTosebinding-proteins)-Fused-Proteins
Express fusion proteins as per the?GST-fused protocol?up to Step 7 (Day 3). All steps in protein purification should be done at 4° C unless otherwise
Measuring-PLD-Activity-In-Vivo
Phospholipase D (PLD) hydrolyzes structural phospholipids like phosphatidylcholine (PC) and phosphatidylethanolamine (PE) into phosphatidic acid (
In-Vivo-Ubiquitination-Assay-by-Agroinfiltration
The ubiquitination/proteasome system is involved in nearly all plant signaling processes. Many signaling components are degraded by the 26S protea
Peripheral-blood-“endothelial-progenitor-cells”
EPC Isolation and Characterization1.?EPCs were obtained by isolating mononuclear cells using Ficoll density-gradient centrifugation of human blood buf
活體生物光學成像技術的應用
作為一項新興的分子、基因表達的分析檢測技術,在體生物光學成像已成功應用于生命科學、生物醫學、分子生物學和藥物研發等領域,取得了大量研究成果,主要包括: 在體監測腫瘤的生長和轉移、基因治療中的基因表達、機體的生理病理改變過程以及進行藥物的篩選和評價等。 1、在體監測腫瘤的生長和轉移
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
Basic-Fluorescent-in-situ-Hybridization-(FISH)
實驗概要Fluorescence ?in situ hybridization method is a kind of physical map drawing method, ?use fluorescent element mark probe, to detect probe and spli
用CRISPR/Cas9對CART細胞進行多重基因編輯(三)
流式細胞術 Flow cytometry?CytoFLEX (Beckman Coulter Inc)?was used to perform fluorescent expression analysis. Cells were harvested on the following day
Conjugation-of-monoclonal-antibodies
Conjugation of monoclonal antibodiesPrelude: You are free to copy and distribute these documents at will--but please do so in their entirety, complete