Introduction to Histology
alubajessabeth
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Mar 23, 2016
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About This Presentation
Histology is the branch of anatomy that deals with the study of tissues in animal and plants.
Slide Content
INTRODUCTION TO
HISTOLOGY
Prof. Redem C. Deligero, MATMRS;MSES
HISTOLOGY
Prof. Redem C. Deligero, MATMRS;MSES
DEFINITION
Histology is the branch of anatomy that
deals with the study of tissues in animal and
plants.
It deals with the structure and its function.
This subject itself intertwines the discipline in cell
biology, biochemistry, physiology and pathology.
Histology is the branch of anatomy that
deals with the study of tissues in animal and
plants.
It deals with the structure and its function.
This subject itself intertwines the discipline in cell
biology, biochemistry, physiology and pathology.
MICROSCOPY
Is the method used in the study of cells
and its structure using microscope.
Major Kind of Microscope
1.Light Microscope – Utilizes light for
illumination.
2.Electron Microscope – Uses an electron
beam.
Is the method used in the study of cells
and its structure using microscope.
Major Kind of Microscope
1.Light Microscope – Utilizes light for
illumination.
2.Electron Microscope – Uses an electron
beam.
LIGHT MICROSCOPE
TRANSMISSION ELECTRON MICROSCOPE
SCANNING ELECTRON MICROSCOPE
3 IMPORTANT PARAMETERS IN
MICROSCOPY
1.Magnification – It is the ratio between the size
of an image produce by the microscope and its
actual size.
2.Resolution – A measure of clarity of an image.
3.Contrast – The ability to visualized a particular
cell structure depending on how different it
looks from an adjacent structure.
MICROSCOPY
1.Magnification – It is the ratio between the size
of an image produce by the microscope and its
actual size.
2.Resolution – A measure of clarity of an image.
3.Contrast – The ability to visualized a particular
cell structure depending on how different it
looks from an adjacent structure.
TISSUE PREPARATION
1.Fixation – treatment of tissue with chemical
agent.
2.Dehydration & Clearing – removal of water from
tissue sample.
3.Embedding – Infiltration of tissue sample with
paraffin.
4.Sectioning – Cutting tissue sample by section into
specific equal increments.
5.Mounting and Staining – Placing the tissue
sample on adhesive glass slides.
1.Fixation – treatment of tissue with chemical
agent.
2.Dehydration & Clearing – removal of water from
tissue sample.
3.Embedding – Infiltration of tissue sample with
paraffin.
4.Sectioning – Cutting tissue sample by section into
specific equal increments.
5.Mounting and Staining – Placing the tissue
sample on adhesive glass slides.
FIXATION
DEHYDRATION & CLEARING
EMBEDDING
SECTIONING
MOUNTING AND STAINING
3 MAJOR CATEGORY OF STAINS
1.Stains that differentiate between acidic
and basic cellular components.
2.Specialized stains that differentiate the
fibrous components of the extracellular
matrix.
3.Metallic salts that precipitate on tissue
forming metal deposits.
1.Stains that differentiate between acidic
and basic cellular components.
2.Specialized stains that differentiate the
fibrous components of the extracellular
matrix.
3.Metallic salts that precipitate on tissue
forming metal deposits.
COMMONLY USED STAINS
1.Hematoxylin – Forms the basophilic
components of the cell.
2.Eosin – Forms the acidophilic
components of the cell.
3.Toluidine Blue – Forms the
metachromatic component of the cell.
1.Hematoxylin – Forms the basophilic
components of the cell.
2.Eosin – Forms the acidophilic
components of the cell.
3.Toluidine Blue – Forms the
metachromatic component of the cell.
HISTOCHEMISTRY
1. Periodic Acid Schiff (PAS) - Is a staining method used to
detect polysaccharides (e.g. glycogen, glycoproteins,
glycolipids and mucins in tissues.
2. Feulgen Reaction - Is used to identify chromosomal
material or DNA in cell specimens.
3. Gomori-Takamatsu - a method for localizing the alkaline
phosphatase enzyme.
4. Mordant - Is a substance used to set dyes on tissue
sections by forming a coordination complex with the dye
which then attaches to the tissue.It may be used for
intensifying stains in cell or tissue preparations.
5. Counterstain - Is a stain with colour contrasting to the
principal stain, making the stained structure more easily
visible.
1. Periodic Acid Schiff (PAS) - Is a staining method used to
detect polysaccharides (e.g. glycogen, glycoproteins,
glycolipids and mucins in tissues.
2. Feulgen Reaction - Is used to identify chromosomal
material or DNA in cell specimens.
3. Gomori-Takamatsu - a method for localizing the alkaline
phosphatase enzyme.
4. Mordant - Is a substance used to set dyes on tissue
sections by forming a coordination complex with the dye
which then attaches to the tissue.It may be used for
intensifying stains in cell or tissue preparations.
5. Counterstain - Is a stain with colour contrasting to the
principal stain, making the stained structure more easily
visible.
HEMATOXYLIN
EOSIN
MASSON'S TRICHOME
ORCEIN'S ELASTIC STAIN
WEIGERT'S ELASTIC STAIN
SILVER STAIN
IRON HEMATOXYLIN STAIN
PERIODIC ACID-SCHIFF
WRIGHT AND GIEMSA STAINS
ADVANCE VISUALIZATION PROCEDURES
1. Hitochemistry
A method if tissue staining that gives
information on the presence and location of
intracellular and extracellular
macromolecules.
2. Immunocytochemistry
It uses flourescenated antibodies &
antiantibodies to exact intracellular and
extracellular localization of macromolecules.
1. Hitochemistry
A method if tissue staining that gives
information on the presence and location of
intracellular and extracellular
macromolecules.
2. Immunocytochemistry
It uses flourescenated antibodies &
antiantibodies to exact intracellular and
extracellular localization of macromolecules.
3. Autoradiography
A method that incorporates radioactive
isotopes into macromolecules which are then
visualized by an overlay of film.
It uses a radio isotopes tritium (
3
H).
A method that incorporates radioactive
isotopes into macromolecules which are then
visualized by an overlay of film.
It uses a radio isotopes tritium (
3
H).
UNITS OF MEASUREMENT
1.Micrometer (µm) – This corresponds to
one-millionth of a meter (10
-6
m )
2.Nanometer (nm) – This corresponds to
one-billionth of a meter (10
-9
m)
3.Angstrom (Å) -This corresponds to one
ten-billionth of a meter (10
-10
m)
1.Micrometer (µm) – This corresponds to
one-millionth of a meter (10
-6
m )
2.Nanometer (nm) – This corresponds to
one-billionth of a meter (10
-9
m)
3.Angstrom (Å) -This corresponds to one
ten-billionth of a meter (10
-10
m)
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