eBook - ePub

Immunophenotyping for Haematologists

Name: Immunophenotyping for Haematologists
Author: Barbara J. Bain, Mike Leach

Principles and Practice

Barbara J. Bain, Mike Leach

Partager le livre

English
ePUB (adapté aux mobiles)
Disponible sur iOS et Android

eBook - ePub

Immunophenotyping for Haematologists

Principles and Practice

Barbara J. Bain, Mike Leach

Détails du livre

Aperçu du livre

Table des matières

Citations

À propos de ce livre

Offers clear and concise instruction on running, reporting and interpreting immunophenotyping studies

Written by two well-known haematology educators and experts on the topic, Immunophenotyping for Haematologists contains an introduction to running, reporting and interpreting immunophenotyping studies. The book offers a unique approach to the topic by putting the focus on clinical and laboratory haematologists who are not routinely involved in running and reporting on immunophenotyping studies.

Immunophenotyping using flow cytometry has become the method of choice in identifying and sorting cells within complex populations, for example, the analysis of immune or neoplastic cells in a blood sample. The text reviews the purpose and principles of immunophenotyping and includes an introduction and explanation of the principles and the role of immunophenotyping. The authors examine immunophenotypic characteristics of the disease groups commonly encountered and identify the features that differentiate malignant cells from normal cells. To enhance understanding, the book contains multiple choice and extended matching questions which integrates immunophenotyping with clinicopathological features and the results of other investigations to mimic everyday practice. This important book:

Provides a concise introduction to running, reporting and interpreting immunophenotyping studies
Contains a list of all the antibody specificities currently widely used in diagnosis and disease monitoring
Presents an ideal reference for use in laboratories, including immunophenotyping laboratories
Aids in the interpretation by covering immunophenotypic characteristics of commonly encountered disease groups
Identifies the features that differentiate malignant cells from their normal counterparts

Written for haematologists working in both laboratory and clinical haematology, Immunophenotyping for Haematologists is a much-needed reference for understanding and interpreting immunophenotyping studies.

Foire aux questions

Comment puis-je résilier mon abonnement ?

Il vous suffit de vous rendre dans la section compte dans paramètres et de cliquer sur « Résilier l’abonnement ». C’est aussi simple que cela ! Une fois que vous aurez résilié votre abonnement, il restera actif pour le reste de la période pour laquelle vous avez payé. Découvrez-en plus ici.

Puis-je / comment puis-je télécharger des livres ?

Pour le moment, tous nos livres en format ePub adaptés aux mobiles peuvent être téléchargés via l’application. La plupart de nos PDF sont également disponibles en téléchargement et les autres seront téléchargeables très prochainement. Découvrez-en plus ici.

Quelle est la différence entre les formules tarifaires ?

Les deux abonnements vous donnent un accès complet à la bibliothèque et à toutes les fonctionnalités de Perlego. Les seules différences sont les tarifs ainsi que la période d’abonnement : avec l’abonnement annuel, vous économiserez environ 30 % par rapport à 12 mois d’abonnement mensuel.

Qu’est-ce que Perlego ?

Nous sommes un service d’abonnement à des ouvrages universitaires en ligne, où vous pouvez accéder à toute une bibliothèque pour un prix inférieur à celui d’un seul livre par mois. Avec plus d’un million de livres sur plus de 1 000 sujets, nous avons ce qu’il vous faut ! Découvrez-en plus ici.

Prenez-vous en charge la synthèse vocale ?

Recherchez le symbole Écouter sur votre prochain livre pour voir si vous pouvez l’écouter. L’outil Écouter lit le texte à haute voix pour vous, en surlignant le passage qui est en cours de lecture. Vous pouvez le mettre sur pause, l’accélérer ou le ralentir. Découvrez-en plus ici.

Est-ce que Immunophenotyping for Haematologists est un PDF/ePUB en ligne ?

Oui, vous pouvez accéder à Immunophenotyping for Haematologists par Barbara J. Bain, Mike Leach en format PDF et/ou ePUB ainsi qu’à d’autres livres populaires dans Medicine et Hematology. Nous disposons de plus d’un million d’ouvrages à découvrir dans notre catalogue.

Informations

Éditeur

Wiley-Blackwell

Année

2020

ISBN

9781119606154

Édition

Sujet

Medicine

Sous-sujet

Hematology

Part 1
Purpose and Principles of Immunophenotyping

Immunophenotyping is the process by which the pattern of expression of antigens by a population of cells is determined. The presence of a specific antigen is recognised by its binding to a labelled antibody. Antibodies can be present in a polyclonal antiserum that is raised in an animal but more often they are well characterised monoclonal antibodies produced by hybridoma technology; a hybridoma is a clone of cells created by the fusion of an antibody‐producing cell with a mouse myeloma cell. Monoclonal antibodies can be labelled with an enzyme or with a chemical, known as a fluorochrome, that under certain circumstances will fluoresce. Immunophenotyping is carried out primarily by flow cytometry or immunohistochemistry. Flow cytometric immunophenotyping is applicable to cells in peripheral blood, bone marrow, body fluids (pleural, pericardial, ascitic and cerebrospinal fluids) and fine needle aspirates. Immunohistochemistry of relevance to haematological disease is applied particularly to trephine biopsy and lymph node biopsy specimens, but also to biopsy specimens from any other tissues where infiltration by haemopoietic or lymphoid cells is suspected.

Flow Cytometric Immunophenotyping

This technique determines cell size, structure (to some extent) and antigen expression. Cells in suspension are first exposed to a combination of fluorochrome‐labelled monoclonal antibodies (or other lectins or ligands) and then pass in a focused stream through a beam of light generated by a laser. Laser‐generated light is coherent (waves of light are parallel) and monochromatic (single wave length/colour). Large multichannel instruments with multiple lasers are used to identify, count, size and otherwise characterise cells that are hydrodynamically focused and pass in a single file through a narrow orifice in a flow cell. The passing of the cell through a light beam leads to both the scattering of light and the excitation of fluorochromes so that they emit a fluorescence signal. Forward scatter (FSC) of light at a narrow angle is detected and measured and is proportional to cell size. Sideways or side scatter (SSC) of light is detected and measured and is proportional to cell granularity and complexity. Antigens expressed on the surface membrane of cells or, with modified techniques, within cells are detected. After ‘permeabilisation’, both cytoplasmic and nuclear antigens can be detected.

For each fluorochrome, a selected laser emits light of a specified wavelength that will be absorbed by the fluorochrome. This leads to excitation of the fluorochrome with subsequent emission of light of lower energy and a longer wavelength as the fluorochrome returns to its basal state; this property is known as fluorescence. The amount of light emitted (the number of photons) is proportional to the amount of fluorochrome bound to the cell. The mean fluorescence intensity of a population indicates the strength of expression of the relevant antigen. The emitted light passes through dichroic mirrors, that is, mirrors that reflect some wavelengths and transmit others, so that it is possible, for example, to reflect SSC for measurement and transmit fluorescence signals to another detector such as a photomultiplier tube (Figure 1.1). The detector produces an electrical signal that is proportional to the amount of incident light. Some commonly used fluorochromes are shown in Table 1.1.

The cells that are studied must be dispersed. For peripheral blood and bone marrow aspirate specimens, it is necessary to exclude mature and immature red cells. This is most simply done by lysing red cells using an ammonium chloride solution. Otherwise red cells and their precursors will appear in scatter plots and interfere with gating leucocyte populations of interest. If assessment of immunoglobulin expression is required, there must also be a washing step to remove the plasma that contains immunoglobulin, which would neutralise the monoclonal lambda‐ or kappa‐specific antibody.

Table 1.1 Commonly used fluorochromes.

Fluorescein isothiocyanate (FITC)

Phycoerythrin (PE)

Allophycocyanine (APC)

Peridinin chlorophyll (PerCP)

Cyanine 5 (Cy5), cyanine 5.5 (Cy5.5) and cyanine 7 (Cy7)

Texas red

Pacific blue

Brilliant violet

Krome orange

Alexa Fluor 488 (AF488)

Alexa Fluor 647 (AF647)

Phycoerythrin‐Texas Red X (ECD)

Phycoerythrin‐cyanine 5 (PE‐Cy5)

Phycoerythrin‐cyanine 5.5 (PE‐Cy5.5)

Phycoerythrin‐cyanine 7 (PE‐Cy7)

The great majority of monoclonal antibodies used in immunophenotyping have been characterised at a series of international workshops and those with the same specificity have been assigned a cluster of differentia...