UseoftheB.D.FACSorCaliburFlowCytometers2
Gating:Gating will allow you to view cells of interest by any combination of criteria that you choose. Gating does not change the intensity value assigned to an event as is the case for changes in voltage or compensation. It simply lets you decide which data to view and which data to ignore or discard. It is important to check that small changes in your gates don't have significant effects on your results or else......阅读全文
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
FACS-Analysis-Using-Peripheral-Blood-Cells
FACS Analysis Using Peripheral Blood CellsCollect blood (75 microliters) into 1ml PBS containing 5 microM EDTA (10 microliters of 0.5 M stock) and mix
Detection-of-Intracellular-Antigens-by-Flow-Cytometry
实验概要Fix and Perm reagents are designed for use with all commercially available flow cytometers. Alignment and compensation should be performed accor
Yeast-Cell-Cycle-by-Flow-Cytometry
ReagentsCold absolute ethanol.0.5 M Na citrate stock (filtered), 50mM diluted stock.10 mg/ml RNase A (Boil 10 mins, cool, filter and store at -20°C).4
Intracellular-Immunofluorescent-Staining-for-Flow-Cytometry
IntroductionA modification of the basic immunofluorescent staining and flow cytometric analysis protocol can be used for the simultaneous analysis of
Flow-Cytometric-Analysis-of-Cell-Cycle
Fixation1) Collect 2 X 106 cells.2) Pellet cells by spinning at 1,000 rpm, 4°C for 5 minutes.3) Resuspend cell pellet in 1 ml of cold PBS.4) Fix cells
HOW-TO-USE-THE-COULTER-COUNTER-TO-COUNT-CELLS
1) Turn on the counter by pulling out the on/off button. You need to do this at least 10 min before use to obtain sufficient vacuum.Usually put 0.2 ml
Guidelines-for-the-Use-of-Analgesics-and-Tranquilizers-in-Laboratory-Animal
What is Anesthesia? Anesthesia is a state of unconsciousness induced in an animal. The three components of anesthesia are analgesia (pain relief), amn
Flow-Cytometric-Analysis-Of-Bcl-Family-members
DescriptionCell Fixation, staining and flow cytometric analysis ProcedureCells (106) were washed twice in FACS buffer (phosphate buffered saline PBS p
以色列X荧光光谱仪XRFCaliburSDD
仪器介绍: XRF-Calibur SDD非常适合于传统的实验室操作,它有完全整合的电脑控制系统。重型设计及制造使得该仪器成为移动实验室的理想选择。 主要特点: 1. 真正实现了快速,准确的检测,直接显示元素的ppm含量或者百分比。 2. 矿石、岩石、矿渣、碎片、土壤、泥土、泥浆等固体和液体物质。
流式细胞仪和流式细胞术指南篇2
核酸插入染料溴化乙锭(EtBr) 和碘化丙啶(PI)能够结合到DNA双螺旋的大沟。4,6-二脒基-2-苯基吲哚(DAPI)和Hoechst染料(有几种常用的)则结合小沟。请注意, 一些染料 (例如碘化丙啶)也会结合到RNA发卡结构形成的沟中,因此如果要做DNA定量,需要用染料和RNA
Flow-Cytometry-of-Fibroblast-Nuclei-for-DNA-content
MaterialsP.I. Solution: 4 mM Na3Citrate (0.118 g/100 mL)30 U/mL RNAseI (43 mg/100 mL)0.1% Triton-X100 (0.1mL/100 mL)50 µg/mL propidium iodide (5 mg/10
Setup-and-use-of-a-twolaser-multiphoton-microscope
Setup and use of a two-laser multiphoton microscope for multichannel intravital fluorescence imagingDavid Entenberg,1 Jeffrey Wyckoff,1 Bojana Gligori
Basic-Theory-and-Use-of-GCMS(一)
BASIC THEORY AND USE OF GC-MSbyDr. Eugenia SobolevaContent1. Introduction.2. GC-MS systems and components.3. Vacuum system3.1. Rotary pump3.2. Di
General-Laboratory-Procedures,-Equipment-Use,-and-Safety-Considerations
A. Storage .The following properties of reagents and conditions are important considerations in processing and storing DNA and RNA. Heavy metals promo
Basic-Theory-and-Use-of-GCMS(二)
For ionisation to take place at all, chemical reaction between the sample and the reagent gas must be exothermic. The grater the heat of the reaction,
Use-of-the-Bradford-Protein-Assay-in-a-Microtiter-Plate-Format
Introduction The Bradford protein assay is a simple procedure for determination of protein concentrations in solutions that depends upon the change in
Combined-Flow-Cytometric-Measurement-of-Two-CellSurface-Antigens2
DNA and RNA Staining6. Stain cells with 7-AAD: i. Resuspend the cells from Step 5 in 0.5 mL of NASS containing 10 µg/mL of 7-AAD. Incubatefor 20 min a
Application-Note:-Qdot®-Nanocrystal-Conjugates-in-Flow-Cytometry
实验概要Researchers today are trying to maximize the information that they get out of flow cytometry experiments by looking at more parameters in a sing
Flow-Sorting-Fibroblasts-with-GFP-and-P.I.
ProtocolWash cells with PBS and trypsinize to a single cell suspension.Count an aliquot on a hemocytometer. Meanwhile centrifuge the cells (e.g. 1000
Intracellular-Immunofluorescent-Staining-for-Flow-Cytometry2
Table 2: Human Cytokines: Intracellular Staining Quick GuideHuman Cytokines: Intracellular Staining Quick GuideHuman CytokineCell SourceActivationIncu
流式细胞仪(Flow-Cytometry)
1 流式细胞仪的概念及其发展历史1.1 流式细胞仪的基本概念 流式细胞仪(flow cytonletry,FCM)是对高速直线流动的细胞或生物微粒进行快速定量测定和分析的仪器,主要包括样品的液流技术、细胞的计数和分选技术,计算机对数据的采集和分析技术等。流式细胞仪以流式细胞术为理论基础,是流体力学、
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
流式细胞仪(Flow-Cytometry)
1 流式细胞仪的概念及其发展历史1.1 流式细胞仪的基本概念 流式细胞仪(flow cytonletry,FCM)是对高速直线流动的细胞或生物微粒进行快速定量测定和分析的仪器,主要包括样品的液流技术、细胞的计数和分选技术,计算机对数据的采集和分析技术等。流式细胞仪以流式细胞术为理论基础,是流体力学、
流式细胞术(Flow-Cytometry,-FCM)
流式细胞术(Flow Cytometry, FCM)是一种在功能水平上对单细胞或其他生物粒子进行定量分析和分选的检测手段,它可以高速分析上万个细胞,并能同时从一个细胞中测得多个参数,与传统的荧光镜检查相比,具有速度快、精度高、准确性好等优点,成为当代最先进的细胞定量分析技术。流式细胞仪(Flow C
Flow-Cell-Assays-with-Microtubules:-Motility/Dynamics-in-Fluorescence
Flow cell assays are very useful for studying microtubule motility, microtubule dynamics, kinetochore-microtubule interactions and action of severing/
Use-of-Nonaqueous-Fractionation-and-Metabolomics-to-Study-Chloroplast-...
Use of Non-aqueous Fractionation and Metabolomics to Study Chloroplast Function in ArabidopsisChloroplasts are the chemical factories of plant cells b
How-to-use-Basic-Local-Alignment-Search-Tool-(BLAST)
DescriptionThe BLAST algorithm was developed as a way to perform DNA and protein sequence similarity searches by an algorithm that is faster than FAST
Use-of-SemiThin-Cryosections-for-Light-Microscopy.
Use of Semi-Thin Cryosections for Light Microscopy.Semi-thin sections can be obtained from frozen blocks of cryoprotected biological material by secti
ex-vivo-expanded-endothelial-progenitor-cells
Cell Culture. 1. Total hPBMCs were isolated from blood of human volunteers by density gradient centrifugation. 2. Cells were plated on culture dishes