IHCProtocolforFr...
实验概要The method provides a IHC protocol for free floating brain sections.实验步骤1. Coronal 30-40 µm sections cut on a freezing microtome. Sections collected into petri dishes containing 1-2ml 0.1M phosphate buffer (PB). Sections can be kept on a shaker at 4oC for several days before commencing the immunocytochemistry. [If left too long, the sections become harder to mount].2. Deactivate endogenous peroxid......阅读全文
Western-Blot-Protocol
一、提取抗原蛋白将提取RNA途中留存的样品,加入150μl 100%酒精充分混匀,静置5min(RT), 2000×g , 4℃离心5min, 吸取上清至新管中, 加入750μl异丙醇, 混匀, 静置10min(RT), 12000×g, 4℃离心10min, 弃上清, 加入1ml 0.3mol/L
Transformation-Protocol-for-Arabidopsis
Transformation Protocol for Arabidopsis – AbbreviatedGerminate seed in pots↓ 4 weeksStreak bacteria onto YM/MinA↓ 2-3 days 28°CSpray/dip bacterial sus
Histone-blotting-protocol
实验概要 Western blot detection of histone proteins. 实验步骤 The following protocol refers to the western blot detection of histone proteins derived from p
Nuclear-Extraction-Protocol
实验概要The procedure presented below describes a method for extracting nuclear from several cell lines of human origin.主要试剂Hypotonic Buffer Solution20 mM
Protocol-for-dsRNA-Synthesis
实验概要 We routinely produce dsRNA by in vitro transcription of a PCR generated DNA template containing the T7 promoter sequence on both ends
BrdU-Labeling-Protocol
实验概要The thymidine analog, 5-bromo-2-deoxyuridine (BrdU),is a common reagent used for cell proliferation assays and for the detection of apoptotic
RNA-Isolation-Protocol
RNA Isolation Protocol(Revised 5-15-2003)Stabilize RNAStart with 15 ml E. coli Culture containing 7.5* 109 cells (OD600= 0.2 Dilute cells or scale up)
Sandwich-ELISA-Protocol
实验概要The Sandwich ELISA measures the amount of antigen between two layers of antibodies (i.e. capture and detection antibody). The antigen to be mea
Cytotoxicity-Assays-Protocol
Cytotoxicity Assays ProtocolCell-mediated cytotoxicity was determined by using a standard microcytotoxicity assay. Briefly, target cells were pelleted
Tissue-Harvest-Protocol
TISSUES TO BE PROCURED(minimally and preferably within 5-8 hours after death):1. Brain2. Liver3. Muscle4. Skin5: Others as the specific case dictatesP
Dot-blot-protocol
实验概要A technique for detecting, analyzing, and identifying proteins, similar to the western blot technique but differing in that protein samples are
Protocol-of-Northern-blot
Protocol of Northern blot质粒的转化和扩增质粒的鉴定目的基因片段的切割3.1样品双酶切(175μl水解体系)DW 115μlBuffer B(10×) 17.5μlBaM H 15μlPst I 17μlDNA(MMP-9) 16μlBSA 4.5μl37℃水浴,3h。3.2
Nucleolar-Isolation-Protocol
We recommend that you first download and read this page as a PDF file. Using that as your guide, you can then follow the protocol below and view a Qui
Western-Blotting-Protocol
实验概要The western blot (sometimes called the protein immunoblot) is a widely used analytical technique used to detect specific proteins in the given s
Yale-Immunofluorescence-Protocol
实验概要We provide a protocol for fixation, immunostaining, and imaging in 384-well Plates.主要试剂Reagents1. 384-well view plates (Aurora)2. HUVEC (pooled, L
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
Phycoerythrin-conjugation-protocol
Phycoerythrin conjugation protocolDavid's method modified from references (2) and (3). I used this method to conjugate a mouse IgG2a monoclonal an
Basic-ELISA-Protocol
实验概要 There are many different types of ELISAs, which can detect the presence of protein in serum or supernatent. One of the most common typ
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
Silver-Staining-Protocol
1x 40min - overnight 50% MeOH, 12% Acetic Acid1x 30min 50% MeOH, 12% Acetic Acid, 0.05% 37% Formaldehyde3x 20min
RNA-Isolation-Protocol
Stabilize RNAStart with 15 ml E. coli Culture containing 7.5* 109 cells (OD600= 0.2 Dilute cells or scale up)Pipet 30 ml of RNAProtect Bacteria Reagen
Microarray-Hybridization-Protocol
Introduction:One microarray set consists of 7 nylon membranes with 2.5 x 7.5 cm dimension. 2304 genes were spotted onto nylon membranes (Schleicher an
IHC,ELISA,WB实验之间的区别
免疫组化、Western、ELISA,是免疫学三大常用工具,分别用于定位,定性和定量。那么,我们今天就来说说这三者之间的差别以及其具体使用的场景。1、IHC中文名称:免疫组化英文名称:Immunohistochemistry简介:是融合了免疫学原理(抗原抗体特异性结合)和组织学技术(组织的取材、固定
IHC原理、操作及注意事项
免疫组织化学(Immunohistochemistry,IHC)是利用抗原与抗体特异性结合的原理,通过化学反应使标记抗体的显色剂(荧光素、酶、金属离子、同位素)显色来确定组织细胞内抗原(多肽和蛋白质),对其进行定位、定性及定量的一项技术。IHC的实验流程和方法总体不难,但做出漂亮的染色结果却不容易,
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
原位免疫PCR的IHC增敏方法
(一)基本原理Sano等(1992)率先利用基因工程的方法表达了A蛋白与链霉亲和素的嵌合体分子获得成功,建立了免疫PCR技术。这是一种新的抗原检测系统,利用细胞工程和基因工程技术,巧妙地将抗原抗体反应的特异性同PCR的敏感性相结合,通过构建单克隆抗体与重组核酸的嵌合体分子,使得利用PCR技术检测蛋白
IHC-增敏实验——滚动循环放大法
实验方法原理滚动式循环放大(rolling circle amplification;RCA)法是一种能够在恒温条件下,使标记有寡核苷酸探针(与组织细胞内的核苷酸无相关性)的抗体(特异性一抗或第二抗)与组织细胞内的抗原结合后,在 DNA 聚合酶的作用下,加入的寡核苷酸进行循环扩增,产生一条扩增的 D
IHC全攻略2:如何制备样品
对于每一项IHC/ICC研究,组织和细胞样本的制备都不可掉以轻心。为了方便孵育,整个组织必须被切成超薄(5-10 μm)的切片,或切成小块用于整体免疫组化(whole mount IHC)。对于ICC实验,在开始染色步骤之前,细胞必须附着在显微镜载玻片或盖玻片上。样本制备也与固定方法密切
Streamlined-DNA-Extraction-Protocol
This method is derived from a procedure developed by Toby Bradshaw and the Poplar Molecular Genetics Cooperative. We have tested the procedure wit
Xenograft-Tumor-Assay-Protocol
1) Determine the number of cells for injection (ie 5´106 ) to determine the number of plates thatwill require trypsinizing (usually a 100% confluent p