DetectionofIntracellularAntigensbyFlowCytometry
實驗概要Fix and Perm reagents are designed for use with all commercially available flow cytometers. Alignment and compensation should be performed according to the manufacturer's instructions. Typical staining and scatter patterns are shown below in Figure 1. Clinical Research Applications: Flow cytometric analysis with monoclonal antibodies has historically been restricted primarily to ......閱讀全文
Coenzyme-A-Detection
實驗概要The experiment provided ?an ?easy, convenient assay to measure the CoA level in a variety of ?biological samples. In the assay, free CoA is specif
Detection-of-Glycoproteins-on-Blot
Detection of Glycoproteins on BlotSource:?Contributed by Sharad Purohit, Paller's LabReagentsSodium acetate Buffer (200mM, pH 5.5): Prepare? a 200
Detection-and-Measurement-of-Radioactivity
Radioactive DecayIsotopes of a given element have nuclei with the same number of protons but different numbers of neutrons. Some isotopes are stable,
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
Detection-and-Measurement-of-Radioactivity
Liquid scintillation countingThe amount of kinetic energy in a beta particle differs from one decay to the next. However, each radioisotope has a typi
Detection-of-Mycoplasma-by-Culture
AimDetection of mycoplasma by culture is the reference method of detection and has a theoretical level of detection of 1 colony-forming unit (cfu). Ho
FACS-Procedures-for-Apoptosis-Detection
Materials:Hoechst?33258?(Sigma B-2883).stock: 10 mg/ml in dH20 (40)working dilution: 500μg/ml (50μl stock + 950μl PBS).7-Amino-actinomycin (Sigma A-94
Bespoke-Metal-Detection-Conveyor-Systems
Many metal detection applications do not fit into the scope of ? standard conveyor systems. For this reason, METTLER TOLEDO SAFELINE are able to p
Protein-detection-onto-PVDF-membranes
2-D PAGE and electroblotting onto PVDF membranes have become widely used techniques for the characterization of proteins. Recent improvements have all
Detection-of-Intracellular-Antigens-by-Flow-Cytometry
實驗概要Fix and Perm ?reagents are designed for use with all commercially available flow ?cytometers. Alignment and compensation should be performed accor
Detection-of-BrdU-Incorporation-in-DNA-Synthesizing-Cells
Detection of BrdU Incorporation in DNA Synthesizing Cells?NOTE:?Bromodeoxyuridine is a known carcinogen. Propidium iodine (PI) is known to be toxic an
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
PCR-Primers-For-Gene-Expression-Detection-or-Quantification
Why PrimerBank?PrimerBank is a public resource for PCR primers. These primers are designed for gene expression detection or quantification (real-time
Cell-death-detection-in-Xenopus-embryos-by-ELISA
Sample preparationWash embryos 1 x in 25% MMRRemove excess bufferAdd 10 volumes "incubation buffer", i.e. 50 μl for 5 embryosLyse the embryos by?gentl
Staining-Procedure-for-Flow-Cytometric-Detection-of-Human-Cyclins
Staining Procedure for Flow Cytometric Detection of Human CyclinsThis is a standard protocol used at Pharmingen for Quality Control testing of the ant
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
Determination-and-Detection-of-Reactive-Oxygen-Species-(ROS),-Lipid-...
Reactive oxygen species or intermediates are formed by the incomplete reduction of oxygen. Organisms living in aerobic environment generate variou
Detection-Of-Cell-Viability-And/Or-Apoptosis-By-Flow-Cytometry-(FACS)
Viable?cells are cells that when allowed to continue beyond the timepoint of examination will stay alive. Besides live and healthy cells, cells in ear
Detection-of-MicroRNA-Heterogeneity-in-Single-Cells-Using-an-Automated
Introduction ?MicroRNA ?(miRNAs) are short (18–24 nucleotides), non-coding RNAs that regulate ?gene expression by both disrupting messenger RNA (mRNA
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-immunocytochemical2
B) TUNEL in situ procedureB.2.1 Materialsproteinase K (pK) (A2), H2O2?, TdT buffer (A1), TdT enzyme (A2), biotinylated dUTP (A2), TB buffer (A1), seru
Methods-for-the-Detection-of-DAminoAcid-Oxidase2
Results and DiscussionNavigationAbstractIntroductionMaterials and MethodsResults and DiscussionReferencesD-Amino-acid oxidase activity was detected in
DualColor-ELISPOT-Assay-for-the-Simultaneous-Detection2
21. Add 100?μL?of developing buffer to all wells?using a multichannel pipette?and incubate at room temperature?for at least 2 h.?22. Wash?the ELISPOT
DualColor-ELISPOT-Assay-for-the-Simultaneous-Detection1
Dual-Color ELISPOT Assay for the Simultaneous Detection of IL-2 and/or IFN- Secreting T CellsINTRODUCTIONThe enzyme-linked immunospot (ELISPOT) assay
Detection-of-Viruses-in-Infected-Plant-Extracts-using-ImmunocapturePCR
?1) Immunocapture stageCoating buffer: 15 mM Na2CO3; 35 mM NaHCO3, and 3 mM NaN3, per liter (pH 9.6).Extraction buffer: (20 mM Tris-HCL (pH 8.0), 138
Methods-for-the-Detection-of-DAminoAcid-Oxidase1
AbstractFour methods (an enzyme activity assay, western blotting, RT-PCR, and northern hybridization) to detect the enzyme D-amino-acid oxidase are de
Detection-of-Viruses-in-Infected-Plant-Extracts-using-ImmunocapturePCR
?1) Immunocapture stageCoating buffer: 15 mM Na2CO3; 35 mM NaHCO3, and 3 mM NaN3, per liter (pH 9.6).Extraction buffer: (20 mM Tris-HCL (pH 8.0), 138
關于細胞凋亡Telemerase-Detection-(端粒酶檢測)的介紹
這是相對來說推出較早,用得較多的一種方法。端粒酶是由RNA和蛋白組成的核蛋白,它可以自身RNA為模板逆轉錄合成端粒區重復序列,使細胞獲得“永生化”。正常體細胞是沒有端粒酶活性的,每分裂一次,染色體的端粒會縮短,這可能作為有絲分裂的一種時鐘,表明細胞年齡、復制衰老或細胞凋亡的信號。研究發現,90%
miRNA-qPCR-Detection-Primer-Set(miRNA檢測試劑盒)實驗說明
一、概述 1、介紹 microRNA(miRNA)是一類有大約22 個核苷酸組成的非編碼小分子RNA,其廣泛存在于真核生物中。miRNA 在個體發育的不同時期及不同組織中有不同的表達模式,都表明了其在發育和分化中起有重大的調控作用。迄今為此,對miRNA 的檢測方法主要有Northe
miRNA-qPCR-Detection-Primer-Set(miRNA檢測試劑盒)實驗說明
一、概述1、介紹microRNA(miRNA)是一類有大約22 個核苷酸組成的非編碼小分子RNA,其廣泛存在于真核生物中。miRNA 在個體發育的不同時期及不同組織中有不同的表達模式,都表明了其在發育和分化中起有重大的調控作用。迄今為此,對miRNA 的檢測方法主要有Northern B