Smolke:Protocols/Western
OverviewBlotting for large V5-tagged proteins in S. cerevisiaeMaterialsY-PER (Pierce)Halt EDTA-free Protease Inhibitor (Pierce)NuPAGE Novex Bis-Tris 4-12% mini gels (Invitrogen NP0321BOX)Prestained protein ladder (NEB P7711S)Protein loading bufferMOPS buffer (Invitrogen NP0001)Nitrocellulose membraneBlotting padsTransfer buffer (Invitrogen NP0006-1)MethanolAnti-V5-HRP antibody (Invitrogen R961-25)Chemiluminescen......阅读全文
Smolke:Protocols/Western
OverviewBlotting for large V5-tagged proteins in S. cerevisiaeMaterialsY-PER (Pierce)Halt EDTA-free Protease Inhibitor (Pierce)NuPAGE Novex Bis-Tris 4
Western-Blotting-Protocols
back to topProtocolStandard vs. Rapid Immunodetection ProceduresThere are two types of protocols for immunodetection: Standard and rapid.Standard vs.
LCM-PROTOCOLS
Slide SectioningParaffin blocks- For DNA analysis:Special LCM processing schedule is followed.The water bath is cleaned using RNAse Zap™, rinsed thoro
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
General-Cloning-Protocols
Large Scale Preps: (See Large scale plsasmid prep protocol for more details)Cultures: Inoculate a 5 mL LB/Amp (50 - 100 µg/mL) culture in early a.m. w
Streptomyces:Protocols/Conjugation
Intergeneric Conjugation and OverlayDescription Transfer of plasmid/cosmid DNA from a host strain, e.g. E.coli ET12567 [pUZ8002], to the recipient str
CGH-Protocols-(四)
CGH Image acquisitionImages were acquired through a Zeiss Axiophot fluorescence microscope using a Plan NEOFLUAR oil objective x63, N.A. 1.25 (Zeiss,
CGH-Protocols-(三)
Hybridizationreagents: labeled tumor and normal-DNA (see protocol Nick translation) salmon sperm DNA, 10 mg/ml (e.g. Promega) human Cot1 DNA, 1 mg/ml
CGH-Protocols-(二)
DNA preparation by cryotom tissue dissectionPreparations/Materials: Cool cryostat down to -20 to -30°C about 3 hours prior to dissection Label eppendo
CGH-Protocols-(一)
Metaphase chromosome preparationMaterials: RPMI 1640 medium fetal calf serum (FCS), 20% Colcemid (e.g. Boehringer Mannheim cell biology reagents, Best
Neutralizing-Bioassay-Protocols
Neutralizing Bioassay ProtocolsIntroductionAntibodies that block binding of cytokines to their specific receptors and neutralize their effects are cri
Streptomyces:Protocols/PCR
Description Polymerase Chain Reaction (PCR) is a method of amplifying a specific DNA target sequence. The cycle involves denaturing the template doubl
Rat-Blood-Collection-Protocols
实验概要The procedure presented below describes a method for collecting rat blood.实验步骤Rat should be fully anesthetized (e.g., unresponsive to toe pinch).1
Streptomyces:Protocols/Transformation-by-Electroporation
Description Transform E.coli cells with plasmid/cosmid DNA using the method of electrophoration (inserting plasmids into E.coli).Approx. Duration:Prep
Streptomyces:Protocols/Spore-Prep
Spore Prep - Inoculating & HarvestingDescription A spore prep is a method of preserving a sporulating strain of Streptomyces. The stock is stored in 2
Protocols-for-LCM-preparation-and-analysis
Protocols for LCM preparation and analysis I. Preparation, LCM and RNA/DNA extraction of Frozen Tissue SectionsA. EmbeddingB. CuttingC. StainingII. Pr
ORNL-MICROARRAY-HYBRIDIZATION-PROTOCOLS
Direct labeling of total RNA with Cy3 and Cy5:A. MATERIALSRNeasy® Mini Kit (Qiagen; Cat # 74106) SuperScript II RT (200U/µL) (Life Technologies; Cat #
DataONE:Protocols/Find-GEO-reuses
Identify reuses of GEO datasetsAimThe aim of this protocol is to collect data on the reuses of datasets in the published literature. This particular p
Red-Blood-Cell-Lysis-Protocols
实验概要BioLegend’s Red Blood Cell (RBC) Lysis Buffer (Cat. No. 420301) has been designed, formulated, and tested to ensure optimal lysis of RBCs in sin
FISH-protocols-for-Drosophila1
.1 RNA Probe Preparation (see Note 1)1. 1.5 mL microcentrifuge tubes or standard 96-well V-bottom microplates.2. RNAse free water.3. T7, T3 or S
FISH-protocols-for-Drosophila2
3. Methods3.1 RNA Probe Preparation1. Different strategies can be used to prepare template DNA for synthesizing antisense RNA probes by in vitro tr
Standard-Protocols-Autoradiography-(35S)
Remove Kodak NTB2 nuclear emulsion from fridge and place at 42oC for around 30-60 mins (until melted).Make up the developer and the fixer and place in
Streptomyces:Protocols/MiniMaxi-Prep
Small Scale Plasmid Isolation (Mini / Maxi Prep)Description A mini prep / maxi prep is used to isolate plasmid or cosmid DNA from bacteria, normally E
Slice-and-Explant-Culture-Protocols-–-Hevner-lab-2002
for axon tracing & cell culture studies in vitro using embyros age E11.5 – E16.5modified from Rubenstein lab and Price lab protocols1. Setupa. 2 hr be
Human-Embryonic-Stem-(ES)-Cell-Protocols——Media-and-Reagents
Serum Free Media for human ES cells on MEFs: can last for 7-10 daysFinal ConcentrationAmount for 250ml Stock solution80% DMEM-F12200ml20% KO Serum Rep
Human-Embryonic-Stem-(ES)-Cell-Protocols——Embryonic-Bodies
Let human ES cells grow until the colonies are large and the cells are pretty piled up - about the time when you would normally split or even a day pa
Western杂交
实验概要本实验介绍了Western杂交的基本流程。主要试剂液氮,提取缓冲液(1 x PBS,10ug/mL Leupeptin,1 mM PMSF,5 mMBenzamidine. 2mM EDTA),转移缓冲液(39mM Glycine,48mM Tris,0.037% SDS,20%甲醇),
Western-Blotting
实验概要Western Blot (AP)主要试剂1. Membrane Blocking buffer:5% Milk 0.05% of Tween 20 PBS2. antibody dilution buffer: PBS 0.05% of Tween20 1.0% Milk(or BSA
Western-Blotting
1. Optional: "Renature" gel- this is thought to permit some refolding of proteins and may be important in finding epitope recognition of monoclonal an
Western杂交
Western杂交l 组织印迹的Western杂交在硝酸纤维素膜上制备组织印迹1.在塑料板上放置两层Whatman 1号滤纸,在滤纸上方放上一张普通纸,然后铺上一层硝酸纤维素膜。2.用双面刀片从植物组织如大豆的茎上切取一块切片(厚度约为1mm)。如果组织表面是湿的,则在Kimwipes纸上