Asemipermanentmountingmediumforimmunofluorescencemicroscopy
A semi-permanent mounting medium for immunofluorescence microscopyMaterials6gm glycerol2.4gm mowiol6ml distilled water12ml Tris buffer 0.2M at pH 8.5MethodWeigh out the glycerol in a 50ml plastic tube and add the mowiol. Stir thoroughly. Add water and leave for 2hr at room temperature. Add the Tris buffer and incubate at approximately 53¡C until the mowiol dissolves, stirring occasionally. Clarify by centrifugation a......阅读全文
A-semipermanent-mounting-medium-for-immunofluorescence-microscopy
A semi-permanent mounting medium for immunofluorescence microscopyMaterials6gm glycerol2.4gm mowiol6ml distilled water12ml Tris buffer 0.2M at pH 8.5M
Fluorescence-Mounting-Medium-(Antifade)
Materials Needed20ml glass scintillation vialSmall stir barFoilGlycerol1X PBSPipets* P-phenylenediamine ( EMD Chemicals Inc. Cat# PX0730)Carbonate-Bic
显微镜技术——光学显微技术
The Light Microscope (House Ear Institute)An explanation of how the light microscope works, how to use it, and how to get optimal results when using i
显微镜技术——荧光显微技术
Immunofluorescencc Microscopy of tissue culture cells (Microscopy and Electronic Imaging Lab)These methods are written for direct staining of filament
免疫荧光
Immunofluorescence Technique (Spector Lab)protocol for immunofluorescence on cells Immunofluorescence Protocol (Walter Steffen)Methanol fixationForma
免疫组织化学
· Double Peroxidase (HRP) Immunohistochemical Labeling of Trypsin-Sensitive Antigens (KPL)· Immunohistochemistry (Tyner lab)This is a
Light-Microscopy
The light microscope, so called because it employs visible light to detect small objects, is probably the most well-known and well-used research tool
ELECTRON-MICROSCOPY
E.M. PROCESSING SCHEDULE - EPOXY RESINFix tissue in 2.5% glutaraldehyde in 0.1M sodium cacodylate buffer at 4oC, for a minimum of 4 hours. Tissue shou
Immunofluroescence-Technique
Fix cells in 2% formaldehyde in PBS/pH 7.4 for 15 min. at 20oC. 2% formaldehyde is made up fresh prior to use by dissolving the appropriate amount of
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
MS-Plant-Tissue-Culture-Medium
Component mg/l in MS mg/l in stock Amount for
MEDIUM-FOR-EMBRYO-RESCUE-(FOR-1-L)
Put 500 mL of distilled water in a 1-L beaker.Add the following:ucrose (6 % final concentration) – 30 gi-inositol (100 mg/L stock is 0.5 g/50 mL) – 10
Microscopy-with-Oil-Immersion
Microscopy with Oil ImmersionPrincipleWhen light passes from a material of one refractive index to material of another, as from glass to air or from a
Immunofluorescence-Microscopy-Protocol
实验概要Immunofluorescence allows the imaging of a specific factor in cells or tissue sections through the use of a specific antibody chemically which i
Phase-Contrast-Microscopy
Phase Contrast MicroscopyPrincipleMost of the detail of living cells is undetectable in bright field microscopy because there is too little contrast b
Immunofluorescence-Microscopy-Protocol
实验概要Immunofluorescence allows the imaging of a specific factor in cells or tissue sections through the use of a specific antibody chemically which i
mccoys-5A-medium是什么
McCoys 5A 培养基适合于多种类型的原代细胞、确立的细胞系以及移植的活检组织的增殖。该培养基适用于多种来源于正常骨髓、皮肤、脾脏、肾、肺、大鼠胚胎以及其他组织的哺乳动物细胞的原代培养。
Immunofluorescence-/-Confocal-Microscopy-Protocol
实验概要Immunofluorescence is a technique used for light microscopy with a fluorescence microscope and is used primarily on biological samples. This tec
Immunofluorescence-/-Confocal-Microscopy-Protocol
实验概要Immunofluorescence is a technique used for light microscopy with a fluorescence microscope and is used primarily on biological samples. This tec
Generic-Fixation-for-Electron-Microscopy
Generic Fixation for Electron MicroscopyThe best way to fix a sample for electron microscopy is to follow a procedure developed and proven by others.
Use-of-Transmission-Electron-Microscopy
Use of Transmission Electron MicroscopyOverviewA protocol describing the use of Zeiss EM9-S transmission electron microscopy is presented. MaterialZe
TUNEL-PROCEDURE-IN-BOVINE-EMBRYOS
Materials8% (w/v) paraformaldehyde stock solution: Dissolve 8 g of powdered paraformaldehyde in 100 ml water. Heat and stir (55-60 C – do not go high
Tunel-Procedure-in-Bovine-Embryos-牛胚胎TUNEL检测凋亡
Materials8% (w/v) paraformaldehyde stock solution: Dissolve 8 g of powdered paraformaldehyde in 100 ml water. Heat and stir (55-60 C – do not go highe
TUNEL-PROCEDURE-IN-BOVINE-EMBRYOS
Materials8% (w/v) paraformaldehyde stock solution: Dissolve 8 g of powdered paraformaldehyde in 100 ml water. Heat and stir (55-60 C – do not go high
CarbohydrateSpecific-Adhesion-of-Intact-Cells-to-Resolved-Glycolipids-on-T
Carbohydrate-Specific Adhesion of Intact Cells to Resolved Glycolipids on TLC PlatesRonald L. Schnaar~Professor, Johns Hopkins University Medical
ImmunohistochemistyFluorescence-Protocol1
MaterialsCytokine-specific Primary Antibodiesunlabeled or biotinylated antigen-affinity purified polyclonal antibodies (R&D Systems ''AF'&
Specimen-Preparation-for-Scanning-Electron-Microscopy
Specimen Preparation for Scanning Electron MicroscopyWe recommend consultation with one of the lab directors before preparing specimens. The methods p
Chlamydomonas-Fixation-for-Transmission-Electron-Microscopy
Chlamydomonas Fixation for Transmission Electron MicroscopySolutions:Chlamydomonas culture medium + 2% glutaraldehyde (5 ml medium + 0.9 ml 25% glutar
Tetrahymena-Fixation-for-Transmission-Electron-Microscopy
Tetrahymena Fixation for Transmission Electron MicroscopyPellet Tetrahymena cells in a clinical centrifuge.OPTIONAL: Suspend cells in HNMK (50 mM HEPE
Fixation-and-Embedding-of-Microtubules-for-Electron-Microscopy
(This procedure can also be used for virtually any material that must be pelleted prior to fixation and thin sectioning)Primary fix:2% glutaraldehyde