Presentation is loading. Please wait.

Presentation is loading. Please wait.

Flow Cytometry at Boston University Medical Campus Introduction to some methods that we offer Yan Deng (X4-5225), Gerald Denis (X4-1371),

Published byAnnabelle Long Modified over 9 years ago

Similar presentations

Presentation on theme: "Flow Cytometry at Boston University Medical Campus Introduction to some methods that we offer Yan Deng (X4-5225), Gerald Denis (X4-1371),"— Presentation transcript:

1 Flow Cytometry at Boston University Medical Campus Introduction to some methods that we offer Yan Deng (X4-5225), ydeng@bu.edu Gerald Denis (X4-1371), gdenis@bu.edu

2 Flow cytometry simultaneously measures and analyzes multiple physical characteristics of single particles, usually cells, as they move in a fluid stream through a beam of light. Any suspended particle between 0.2 and 50μM is suitable. Larger particles, solid tissue or clumps of cells must be disaggregated to be analyzed. Examples: lymphocytes, protozoa, micron beads, chromosomes Definitions

3 The particles in the fluid stream scatter incident light, which reveals internal properties, size and granularity. The particles also fluoresce; they emit laser light at the interrogation point; this light is picked up by detectors arrayed at a different angle to detectors of scattered light. Definitions

4 fluidics optics electronics

5 Fluidics sample flow cell laser waste ~2 x 10 5 to 1 x 10 7 cells/ml sheath fluid

6 Electronics eventFSC (size) SSC (granularity) FL1 (green) FL2 (yellow) FL3 (red) FL4 etc 150030063884020- 22001002458550- 360080030070030- digitize

7 Fluidics Purpose of the fluidics system: 1.Transport particles in a fluid stream to the laser beam to be interrogated 2. Position the sample core in the center of the laser beam sheath fluid sample fluid ‘hydrodynamic focusing’ single file particles ● low flow rate ● narrow sample core ● high resolution ● high flow rate ● wide sample core ● low resolution

8 Fluidics Concerns 1.Shear rates for cells: check after you complete a run to ensure that the cells are intact. 2. Larger tips are needed for cell sorting.

9 Optics Excitation is accomplished by lasers that emit light at specified wavelengths. The atomic properties of the excitation media define this wavelength for a particular laser. The laser beam is focused on the sample core; lasers must be fixed in place. This is the most common and versatile wavelength for excitation of fluorochromes. Argon blue lasers emit light at 488 nm.

10 Fluorescein (FITC) Hoechst 33258Texas Red Propidium iodide (PI) Laser light must overlap with excitation wavelength

11 Optics Filters resolve overlapping wavelengths of emitted light Longpass filter: transmits light of longer than or equal to a specific wavelength Shortpass filter: transmits light of shorter than or equal to a specific wavelength Bandpass filter: transmits light only within a narrow range of wavelengths

12

13

14 Excitation of Texas Red is not optimal with 488 nm laser

15 http://probes.invitrogen.com/resources/spectraviewer/ http://www.bdbiosciences.com/spectra/ For more information

16 Electronics The electronic system: 1.quantifies the voltage pulse 2.converts analog signals to digital values 3.performs compensation 4.transfers data to the computer for analysis.

17 Adjusting the voltage of the PMT helps to optimize capture of desired populations Electronics – Photomultiplier Tubes (PMTs)

18 Electronics - Amplifiers Amplifiers are of two types: linear or logarithmic Linear amplification is typically used with scatter. Logarithmic amplification is typically used with fluorescence. DNA content (Linear detection) DNA content (Log detection)

19 Electronics Threshold is the minimum pulse height above which a signal will be processed electronically.

20 Electronics When a threshold value is defined, only signals with intensities greater than or equal to the value are recorded. Adjustment of blood immunophenotype to exclude debris beforeafter

21 Fluorescence

22 Fluorescence intensity is proportional to the number of binding sites of the fluorescent compound, or “fluorochrome”. Remember, when labeling live cells, to keep the experiment at 4 0 C, because receptors are internalized and recycled, leaving their fluorochromes behind.

23 Immunophenotyping negative stain positive stain

24 Cluster of Differentiation antibody specificity CD3Pan-T lymphocytes CD4T helper/Inducer CD5T cells, subset B cells CD11bMonocytes, granulocytes, NK/T cells CD19B cells CD20B cells CD25 Il-2R, Tac IL-2 receptor, Activated T cells, B cells, NK cells, monocytes CD34 Progenitor cells CD69 Early activation antigen on T, B and NK cells

25 Immunophenotyping Two-color fluorescence of lymphocytes 48% 44% 7% 1% CD19-FITC CD3-PE Note the experiment-specific definition of the “negative” population

26 Fluorescence Multicolor analysis Spectral overlap

27 Compensation To correct for emission spillover of FITC signal (normally detected in the FL1 channel) into the FL2 channel (which detects PE), it is necessary to use filters or electronic compensation or both. UncompensatedOptimal

28 Compensation BeforeAfter Multicolor immunophenotyping

29 Data presentation formats

30 Gates

31

32 The uses of gates for cell sorting

33 Some applications Multiparameter sorting Cell cycle kinetics

34 Some applications DNA content for cell cycle / apoptosis Immune system activation

Download ppt "Flow Cytometry at Boston University Medical Campus Introduction to some methods that we offer Yan Deng (X4-5225), Gerald Denis (X4-1371),"

Similar presentations

Research Techniques Made Simple: Flow Cytometry Richard R

Research Techniques Made Simple: Flow Cytometry Richard R
Slide 1, 4/12/2015 of DNA.ppt  Purdue University Cytometry Laboratories DNA1.ppt.

Slide 1, 4/12/2015 of DNA.ppt  Purdue University Cytometry Laboratories DNA1.ppt.
1 2 3 * Flow = cells in motion * Cyto = cell * Metry = measure * Measuring properties of cells while in a fluid stream * Flow Sorting * Sorting (separating)

1 2 3 * Flow = cells in motion * Cyto = cell * Metry = measure * Measuring properties of cells while in a fluid stream * Flow Sorting * Sorting (separating)
What is Flow Cytometry? Introduction to Flow Cytometry

What is Flow Cytometry? Introduction to Flow Cytometry
What is Flow Cytometry? Flow Cytometry uic Introduction to Flow Cytometry IGC Workshop Multicolor Flow Cytometry IGC – April 28, 2010 Adapted from Holden.

What is Flow Cytometry? Flow Cytometry uic Introduction to Flow Cytometry IGC Workshop Multicolor Flow Cytometry IGC – April 28, 2010 Adapted from Holden.
Intro to Flow Cytometry James Marvin Director, Flow Cytometry Core Facility University of Utah Health Sciences Center Office 801-585-7382 Lab 801-581-8641.

Intro to Flow Cytometry James Marvin Director, Flow Cytometry Core Facility University of Utah Health Sciences Center Office Lab
Avoiding bleed-through artifacts on the confocal microscope Fluorescent dyes are molecules that, when exposed to light of a specific range of wavelengths,

Avoiding bleed-through artifacts on the confocal microscope Fluorescent dyes are molecules that, when exposed to light of a specific range of wavelengths,
Welcome IQAC at DHVI CD4 Immunophenotyping for HIV Monitoring Flow Cytometry.

Welcome IQAC at DHVI CD4 Immunophenotyping for HIV Monitoring Flow Cytometry.
Center of Excellence in Cancer Research Principles of flow cytometry

Center of Excellence in Cancer Research Principles of flow cytometry
CHAPTER 37 MLAB 1415 HEMATOLOGY JOANNA ELLIS, MLS(ASCP) Optical Light Scatter and Flow Cytometry.

CHAPTER 37 MLAB 1415 HEMATOLOGY JOANNA ELLIS, MLS(ASCP) Optical Light Scatter and Flow Cytometry.
Advancements in FACS analyzers optical design leads to greater functionality and a smaller footprint. INTRODUCTION In the past decade, instrumentation.

Advancements in FACS analyzers optical design leads to greater functionality and a smaller footprint. INTRODUCTION In the past decade, instrumentation.
COMPENSATION By: Ronald Mathieu. Compensation Why do we need compensation? –1) Because of long emission spectrum of dyes like FITC and PE.

COMPENSATION By: Ronald Mathieu. Compensation Why do we need compensation? –1) Because of long emission spectrum of dyes like FITC and PE.
DCFH-DA DCFH-DA DCFH DCF H O 2 2 2 2 Oxidative Burst.

DCFH-DA DCFH-DA DCFH DCF H O Oxidative Burst.
Page 1 © 1988-2006 J.Paul Robinson, Purdue University BMS 602 LECTURE 9.PPT BMS 631 - LECTURE 10x Flow Cytometry: Theory Bindley Bioscience Center Purdue.

Page 1 © J.Paul Robinson, Purdue University BMS 602 LECTURE 9.PPT BMS LECTURE 10x Flow Cytometry: Theory Bindley Bioscience Center Purdue.
FLOW CYTOMETRY Dr. MOHAMMED H SAIEMA LDAHR KAAU FACULTY OF APPLIED MEDICAL SCIENCES MEDICAL TECHNOLOGY DEPT. 2 ND YEAR MT INSTROMINTATION EXT 21060.

FLOW CYTOMETRY Dr. MOHAMMED H SAIEMA LDAHR KAAU FACULTY OF APPLIED MEDICAL SCIENCES MEDICAL TECHNOLOGY DEPT. 2 ND YEAR MT INSTROMINTATION EXT
FLOW CYTOMETRY Dr. MOHAMMED H SAIEMA LDAHR KAAU FACULTY OF APPLIED MEDICAL SCIENCES MEDICAL TECHNOLOGY DEPT. 2 ND YEAR MT INSTROMINTATION EXT 21060.

FLOW CYTOMETRY Dr. MOHAMMED H SAIEMA LDAHR KAAU FACULTY OF APPLIED MEDICAL SCIENCES MEDICAL TECHNOLOGY DEPT. 2 ND YEAR MT INSTROMINTATION EXT
Introduction to the Principles of Flow Cytometry

Introduction to the Principles of Flow Cytometry
Overview What is flow cytometry? Development of flow cytometry Components of Flow Typical applications Flow data.

Overview What is flow cytometry? Development of flow cytometry Components of Flow Typical applications Flow data.
Flow Cytometry Basics James Marvin Director, Flow Cytometry Core Facility University of Utah Health Sciences Center Office 801-585-7382 Lab 801-581-8641.

Flow Cytometry Basics James Marvin Director, Flow Cytometry Core Facility University of Utah Health Sciences Center Office Lab
FACSCalibur Training General Information The FACSCalibur is a useful analysis tool. The instrument has 2 lasers- 488 (primary) and 633 (secondary) that.

FACSCalibur Training General Information The FACSCalibur is a useful analysis tool. The instrument has 2 lasers- 488 (primary) and 633 (secondary) that.

Similar presentations

Ads by Google