PreparationandStainingofParaffinSections
I. Fixation and Processing of Tissue for Paraffin SectionsA. Fixation of Tissues in 10% Neutral Buffered FormalinSacrifice animal by prescribed and approved euthanasia techniques. Tissues to be fixed and processed should be cut to a size no larger than 3mm thick. Let tissues fix in 10% formalin at room temperature for 8 hours but not to exceed 24 hours. For small rodent tissue, it is recommended to fix tissues for 4-......阅读全文
Tissue-preparation-protocol-for-ChIP
实验概要This protocol describes how chromatin is prepared from tissue, which can subsequently be used for chromatin immunoprecipitation (ChIP). It is re
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
Maxiprep-preparation-of-Plasmid-DNA
实验概要The PureLink™ HiPure Plasmid DNA Maxiprep Kit allows purification of 500–850 μg of high-quality plasmid DNA from 100–200 mL overnight E. coli cu
胚胎和成年斑马鱼眼情的组织学准备
INTRODUCTIONThis protocol describes the histological preparation of embryonic and adult zebrafish eyes. The methods described here can be easily adapt
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
骨组织βgal免疫染色实验技术方法
ß-gal Staining:Reagents:0.1M Phosphate Buffer (pH 7.3):0.1M Sodium Phosphate monobasic115ml0.1M sodium phosphate dibasic385mlTotal Volume500 mlFix sol
Immunofluorescent-Staining-of-Drosophila-Larval-Brain-Tissue
实验概要The Drosophila larval brain is a well-established model for investigating the role of stem cells in development. Neuroblasts (neural stem cells)
Cell-Cycle-Staining-ProtocolDAPI
1. Harvest cells- wash 2X in PBS to get rid of serum proteins. 1200rpm, 5 min2. Resuspend pellet (up to 3x106 cells) in 1.2 ml PBS (Ca and Mg free).3.
FIXATION-and-DNA-Staining-for-Cell-Cycle-Analysis
BackgroundThis method of DNA staining utilizes ethanol to fix the cells and permeabilize the membrane, which allows the dye (Propidium Iodide) to ente
Protocol-for-intracytoplasmic-staining-of-cytokines-for-FACS-analysis
DescriptionProtocol for intracytoplasmic staining of cytokines for FACS analysis Procedure1) Prepare spleen, lymph node or T cell clone cells as singl
Immunofluorescent-Staining-of-Drosophila-Larval-Brain-Tissue
INTRODUCTIONThe Drosophila larval brain is a well-established model for investigating the role of stem cells in development. Neuroblasts (neural stem
细菌的芽孢染色(spore-staining)
实验原理细菌的芽胞具有厚而致密的壁,透性低,不易着色,若用一般染色法只能使菌体着色而芽胞不着色(芽孢呈无色透明状)。芽孢染色法就是根据芽孢既难以染色而一旦染上色后又难以脱色这一特点而设计的。所有的芽孢染色法都基于同一个原则:除了用着色力强的染料外,还需要加热,以促进芽孢着色。当染芽孢时,菌体也会着色
TEM-Specimen-Preparation:Preparative-Techniques-for-the-TEM
For routine transmission electron microscopy (TEM), it is generally accepted that specimens should be thin, dry and contain molecules which diffract e
流式细胞仪技术专辑
最方便的实验干货查询工具微信扫码进入「丁香实验」小程序编辑: 呜咽分享到: Flow Cytometry Analysis (Springer Lab, Harvard University)Flow cytometry employs instrumentation that scan
ImmunohistochemistyFluorescence-Protocol1
MaterialsCytokine-specific Primary Antibodiesunlabeled or biotinylated antigen-affinity purified polyclonal antibodies (R&D Systems ''AF'&
DAPI-Counterstaining-Protocols
实验概要The blue-fluorescent DAPI nucleic acid stain preferentially stains dsDNA; it appears to associate with AT clusters in the minor groove. Binding
Detection-by-TUNEL-labeling
In Situ Cell Death (Apoptosis) Detection by TUNEL labelingby Boehringer Mannheim (Catalog No. 1684809), modified by Josiah N. Wilcox,José C. Rodriguez
细胞遗传学——比较基因组杂交(CGH)
· Comparative Genomic Hybridization (CGH) CGH is a molecular Cytogenetic method of screening a tumor for genetic changes. The alterations are
E.Z.N.A.®-Protocol-for-ParaffinEmbedded-Tissue
实验概要The E.Z.N.A.® Tissue DNA Kit provides a rapid and easy method for the isolation of genomic DNA for consistent PCR and Southern analysis. Up to
DNAse-posttreatment-for-nuclear-antigens
Rationale: The use of DNAse to improve nuclear antigen staining has been published long before the AR era 1, 2.DNAse treatment is currently suggested
DNA电泳
DNA电泳(主要内容如下) Preparation of Agarose Gel and Electrophoresis Extraction of DNA From Agarose Gel Extraction of DNA from Acrylamide Gels DNA Marker
Preparation-of-Broth-and-Plates,-etc.
Recipes: 1) LB BrothMake 16 gm of LB Broth Base (Gibco #M27800C) up to 800 ml in ddH2O. Swirl to dissolve, then add 110 µl of 10 N NaOH. Autoclave. 2
Large-Scale-Tubulin-Preparation——2
III. Pouring a 1L Phosphocellulose (PC) ColumnResin: Whatman P11 Cellulose Phosphate -- fibrous cation exchanger(1 gram of PC swells to about 4 ml pac
Preparation-of-Rat-Liver-Cell-Cytosol
These protocols should yield enough cytosol and organelles for 1-200 MT/Organelle motility assays.Solutions and Reagents Freshly removed or flash fro
Preparation-of-Agarose-Gels-for-DNA-separations
Weigh out the desired amount of agarose and place in an Erlenmeyer flask with a measured amount of electrophoresis buffer, e.g. for an 0.8% gel, add 0
Preparation-of-Segmented-and-Polarity-Marked-Microtubules
Segmented and polarity-marked microtubules are very useful for many different types of in vitro assays. Segmented microtubules are microtubules with a
Preparation-of-Mitochondria-from-Rat-Liver
Preparation of Mitochondria from Rat LiverRat liver is an ideal source for functional intact mitochondria for a number of reasons. We use Sprague-Dawl