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
Preparation-of-Segmented-and-Polarity-Marked-Microtubules
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Specimen-Preparation-for-Scanning-Electron-Microscopy
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Staining-Procedure-for-Flow-Cytometric-Detection-of-Human-Cyclins
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Table 2: Human Cytokines: Intracellular Staining Quick GuideHuman Cytokines: Intracellular Staining Quick GuideHuman CytokineCell SourceActivationIncu
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AP Buffer:100 mM Tris-HCl, pH 9.5100 mM NaCl10 mM MgCl2PTM:PBS0.1% Tween-202 mM MgCl2Since this is generally done in conjunction with lacZ staining, e
Betagal-staining-of-eukaryotic-cells-in-vitro
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银染(silver-staining)操作规程
实验原理:在碱性条件下,用甲醛将蛋白带上的硝酸银(银离子)还原成金属银,以使银颗粒沉积在蛋白带上。染色的程度与蛋白中的一些特殊的基团有关,不含或者很少含半胱氨酸残基的蛋白质有时候呈负染。银染的详细机制还不是非常清楚。 试剂:乙醇、冰醋酸、乙酸钠、硫代硫酸钠、硝酸银、碳酸钠、甘氨酸或EDTA.Na
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ASENSITIVE-METHOD-FOR-DETECTION-OF-APOPTOSIS-BY-SINGLE-LASER-FLOW-CYTOMETRY
MATERIALS:1. 1 X PBS (PBSAz, 1 X PBS, e.g., Irvine Scientific, CA, containing 2% newborn calf serum and 0.1% sodium azide)2. 7-Amino-actinomycin D (7-
Detection-of-apoptotic-process-in-situ-using-immunocytochemical
1. INTRODUCTION Apoptosis was observed from invertebrates to lower and higher verterbrates, and intervenes both in physiological and in pathological
Multicolour-3DFISH-in-vertebrate-cells5
Author NotesAfter the fourth round of DOP amplification the probe quality is considerably reduced.Use the low stringency cycles only in case you start
Protocol-to-Count-Cell-Number-of-Preimplantation-Embryos
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细胞组分和细胞器——细胞器分离
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Preparation-of-Luciferin-for-In-Vitro-and-In-Vivo-Bioluminescent-Assays
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Preparation-of-phage-particles-from-phage-vectors
Pick up one phage vectors-containing colony with a sterile loop and put into 10 ml 2xTY + 10 µg/l tetracycline.Shake at 200 rpm and 37 °C untill the
Preparation-of-Luciferin-for-In-Vitro-and-In-Vivo-Bioluminescent-Assays
实验概要Reagent for immunoassay, ligand binding assay and ligand receptor assay in which luciferin is covalently bonded to a molecule having biological
Preparation-Of-Ciliated-Protozoa-For-Scanning-Electron-Microscopy
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Preparation-of-bOGDOPG-mixed-micelles
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Preparation-Of-Peripheral-Blood-Cells-For-Chromosome-Analysis
实验概要Lymphocytes are differentiated cells which normally do not undergo subsequent cell divisions. By culturing lymphocytes in the presence of a mito
Adrenal-chromaffin-granule-(chromaffin-vesicle)-preparation
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Human-Peripheral-Blood-Mononuclear-Cell-Preparation
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Preparation-of-Yeast-DNA-Embedded-in-Agarose-Plugs
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Preparation-of-Conventional-Actin-from-Skeletal-Muscle
Modified from Spudich & Watt, 1971, JBC 246:4866.1. Mix 20 ml buffer G with each gm of muscle acetone powder. Extract with stirring on ice for 30 min.
Preparation-of-Luciferin-for-In-Vitro-and-In-Vivo-Bioluminescent-Assays
实验概要Reagent for immunoassay, ligand binding assay and ligand receptor assay in which luciferin is covalently bonded to a molecule having biological
Column-Method-for-Lambda-Phage-DNA-Preparation
Purpose:Mini-prep method for lambda phage DNA purification from lysates.Time required:4 hours once the lysate is in handSpecial supplies required:BioR
Method:-Preparation-of-Lymphocyte-Cell-Pellet-for-Storage
Method: Preparation of Lymphocyte Cell Pellet for StorageJune 10, 1990Rosalie VeilePurpose:Following propagation to 1 X 108 cells, lymphoblastoid cell
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Whole-mount-antibody-staining-ofzebrafish-embryos-formarkers-ofsegmentation
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DAPI-Nucleic-Acid-Stain
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RNA-Purification-from-1020-mg-Paraffinembedded-Tissue
实验概要The E.Z.N.A.® SQ Tissue RNA Kit is designed for isolating total RNA from animal tissue and cultured cells. The solution based system can be easi