PreparationandStainingofFrozenTissueSections
I. Preparation of Frozen Sections for SectioningMaterials neeed:2-methylbutane (isopentane)Liquid NitrogenDry icePeel-Away?/sup> base moldsFrozen tissue matrix (OCT?/sup> or Cryomatrix?/sup>)Long forcepsNecropsy toolsSuperfrost Plus slidesLabel base mold and partially fill the mold with frozen tissue matrix.Sacrifice animal by prescribed and approved euthanasia techniques.Remove desired tissues, trim and cut......阅读全文
实验室荧光显微镜的标本制作方法与正确步骤
一、 玻片及盖玻片(Slide and Coverslips) 玻片及盖玻片质量必需很好而没有荧光,玻片厚度≦1.0mm 者便可用,玻片之清洗,必需以中性清洁剂洗净,再浸于含有3%HCl 之乙醇12~24 小时,然后再贮存于纯酒精。要用时,以清洁纱布擦净或火焰烘干。用完后可浸于水中,移去封
Nested-RTPCR-for-Hepatitis-C-from-Paraffin-Sections
RNA Extraction from Histologic SectionsUnstained 4 µm thick sections of formalin fixed paraffin embedded liver biopsies were transferred from glass sl
Determining-if-anti...
实验概要We provide IHC and WB tips and procedure using alkaline phosphatase to determine if the antibody binds only phosphorylated forms of the target
The-UnderAgarose-Migration-Assay
overviewThe Under-Agarose assay is a useful method for observing the response of a cell population to one or more chemoattractant sources. The behavio
TISSUE-CULTURE-STOCK-SOLUTIONS-AND-MEDIA
MS MEDIUM FOR ARABIDOPSISTo 990 ml H2O add: Sucrose ........... 10.0 g MOPS .............. 0.5 g Agar .............. 8.0 g Adjust pH to 5.7
MS-Plant-Tissue-Culture-Medium
Component mg/l in MS mg/l in stock Amount for
Apoptotic-DNA-fragmentation-and-tissue-homeostasis
Apoptotic cell death can be triggered by many different cellular stimuli, resulting in activation of apoptotic signaling pathways including caspases (
TISSUE-FIBROBLAST-CULTURES-FOR-CHROMOSOME-ANALYSIS
实验概要 Skin tissue may be used for chromosome analysis in special cases when the results from peripheral blood are inconclusive, e.g. suspect
Immunofluorescence-Microscopy-of-tissue-culture-cells
Immunofluorescence Microscopy of tissue culture cellsThese methods are written for direct staining of filamentous actin with bodipy FL-phallicidin and
Dissociation-of-Cells-from-Primary-Tissue
实验概要A common method to obtain single cell suspensions from primary tissue is enzymatic disaggregation. Expose the cells to enzymes for a minimal am
Tissue-Culture-Methods1
I. TYPES OF CELLS GROWN IN CULTURETissue culture is often a generic term that refers to both organ culture and cell culture and the terms are often us
Tissue-Culture-Methods2
IV. MAINTENANCECultures should be examined daily, observing the morphology, the color of the medium and the density of the cells. A tissue culture log
Eccles:Protein-Lysates-from-Tissue
Cell Lysis Buffer5mL 0.1M Tris HCl pH 8 (10mM)0.44g NaCl (150mM)0.02g EDTA (1mM)0.5mL nonidet P40 (1% w/v)0.05g SDS (0.1% w/v)Make up to 50mL with MQH
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
HP-Tissue-DNA-Maxi-Protocol
实验概要The E.Z.N.A.® HP Tissue DNA Maxi Kit is designed for efficient recovery of genomic DNA up to 60 kb in size from up to 2 grams of tissue samples.
HP-Tissue-DNA-Midi-Protocol
实验概要The E.Z.N.A.® HP Tissue DNA Midi Kit is designed for efficient recovery of genomic DNA up to 60 kb in size from up to 500mg of tissue samples.
Method:-Lymphoblastoid-Cell-Lines-from-Frozen-Whole-Blood
Method: Lymphoblastoid Cell Lines from Frozen Whole BloodMay 31, 1990Rosalie VeilePurpose:Blood Samples can be stored frozen as a backup in case an LC
Fungal-Midi-DNA-Kit-Protocol-for-Fresh/Frozen-Specimens
实验概要This protocol is suitable for most fresh or frozen tissue samples allowing more efficient recovery of DNA. However, due to the tremendous variat
与骨骼相关的组织学实验技术方法
Embedding Bones for Frozen Section:Fill an ice bucket with dry ice pellets and place a 500ml beaker in the middle.Put approximately 200ml of 2-MethylB
immunofluorescence-of-rabbit-antimurine-leptin-by-Peprotech
实验概要The following protocol provides a method of immunofluorescence of rabbit anti-murine leptin by Peprotech.实验步骤The following protocol used Trichur
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
TUNEL-labeling
In Situ Cell Death (Apoptosis) Detection by TUNEL labelingby Boehringer Mannheim (Catalog No. 1684809), modified by Josiah N. Wilcox andJosé C. Rodrig
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
Easy-YAC-Preparation-Method
YAC TRANSFORMATION OF C. ELEGANS USING TOTAL YEAST GENOMIC DNA[This method is described in The Worm Breeder's Gazette (1997) A. Davies and J. Shaw
Preparation-of-Sonicated-Human-DNA
Purpose:To break up high molecular weight human placental DNA into fragment sizes of 500 bp or less which can be used as competitor DNA in Southern an
Preparation-of-tubulin2
DAY 2: Cycling preparation of MT protein.Keep the brains in an evacuated plastic ziplock bag buried in ice from the time of slaughter during transport
Midiprep-preparation-of-Plasmid-DNA
实验概要The PureLink™ HiPure Plasmid DNA Midiprep Kit allows purification of 100–350 μg of high-quality plasmid DNA from 15–25 mL overnight E. coli cul
Large-Scale-Tubulin-Preparation
Tubulin is purified from bovine/porcine brain by two cycles of polymerization/depolymerization followed by removal of copurifying proteins on a phosph
Preparation-of-Lactobacillus-Competent-Cells
OverviewInstructions on how to prepare Lactobacillus plantarum competent cells before electrotransformation.MaterialsMRS mediaCulture of L. plantarum
Preparation-of-nucleic-acid-probes
Preparation of nucleic acid probesIn standard nucleic acid hybridization assays the probe is labeled in some way. Nucleic acid probes may be made as s