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INTRODUCTION TO ELECTRON MICROSCOPY,
TRANSMISSION ELECTRON MICROSCOPY IN DETAIL-
INCLUDING FIXATION, PROCESSING & SECTIONING
OF SPECIMENS FOR TEM STUDY
DR. MOUNIKA. S
Post graduate student
Department of Oral Pathology & Microbiology
SRM Dental College,
Ramapuram, Chennai, India
CONTENTS
 APPLICATIONS OF TEM
ADVANTAGES &
DISADVANTAGES OF TEM
 SAMPLE PREPARATION
 FIXATION
 PROCESSING
 SECTIONING
 STAINING
 INTRODUCTION
 COMPONENTS OF ELECTRON
MICROSCOPE
 TRANSMISSION ELECTRON
MICROSCOPY
 PRINCIPLES OF TEM
 ELECTRON INTERACTION IN
TEM
INSTRUMENTATION- VACCUM,
ELECTRICAL, MICROSCOPE
COLUMN& ELECTRON OPTICS 2
 Microscope magnifies the image of the object so that we can visualize the
smallest particles.
 Wavelength in light microscopy is 300-700 nm
 During the first part of the twentieth century, the wave like property of the
electron was demonstrated, and subsequently this has been utilized in
electron microscope (EM).
 Max Knoll & Ernest Rusker- DISCOVERED EM
INTRODUCTION
v According to De Brogle's formula, λ=h/mv
v λ is wavelength, h = 6.626 × 10−34 (Planck’s constant), m = mass
and v = speed of the electron.
v Increase in speed of electron can decrease the wavelength-
better resolution.
v Wavelength in EM- 0.2 nm.
v EM images provide key information on the structural basis of
cell function and of cell disease
PROPERTIES OF ELECTRON
Electrons have shorter wavelength and
provide very high-resolution capacity.
It is easy to manipulate
Electron gives high brightness
Electron beam interacts strongly with
matter
ELECTRON
MICROSCOPY
TEM
BFTEM DFTEM EFTEM ED
SEM AEM STEM
COMPARISON BETWEEN LIGHT AND
ELECTRON MICROSCOPES
COMPONENTS OF ELECTRON MICROSCOPE
1. Electron source
2. Sample
illumination
3. Objective lens
4. Intermediate and
projector lenses
5. Detectors
Electron Source
Electron gun
generates the beam
of electrons.
It consists of a: (a)
Tungsten filament
(b) Wehnelt cylinder
(cathode shield) (c)
Anode plate
TRANSMISSION ELECTRON MICROSCOPY&
PRINCIPLES
12
1 3 5
6
4
2
LIGHT FROM LIGHT
SOURCE
MAGNIFIED IMAGE
BY OBJECTIVE
LENS
BRIGHTELY
ILLUMINATED
FIELD OF VISION
PASSES THROUGH
TRANSPARENT OBJECT
VIRTUAL IMAGE BY
OCCULAR LENS
LIGHT MICROSCOPY
13
1 3 5
6
4
2
COUNTERPART OF
LIGHT
MICROSCOPE
50% INCIDENT
ELECTRONS
THROUGH ULTRA
THIN SECTIONS
2D IMAGES ARE
SEEN
PASSAGE OF HIGH
VELOCITY HOMOGENOUS
ELECTRONS
EMERGENT BEAM
FOCUSSED TO EML
TRANSMISSION ELECTRON MICROSCOPY
ELECTRON INTERACTION IN TEM
INSTRUMENTATION OF TEM
THE VACCUM
SYSTEM
THE
ELECTRICAL
SYSTEM
MICROSCOPE
COLUMN &
ELECTRON
OPTICS
THE VACCUM SYSTEM
17
 Electron beam should be inside a vacum chamber for 2 reasons:
1. To prevent gas molecules colliding with electrons
2. Prevents oxidation of tungsten molecules thus, increasing
longevity
 A series of pumps are employed it includes,
MECHANICAL
ROTARY
PUMP 1x10-
2Pa
DIFFUSION
PUMP 1X10 -
5Pa
TURBO
MOLECULAR
PUMP
ION
PUMP 1x10-
7Pa
THE ELECTRICAL SYSTEM
18
HIGH TENSION
UNIT
LENS CURRENT
SUPPLY UNIT
VOLTAGE & LENS
CURRENT
STABILISER UNIT
MICROSCOPE COLUMN &ELECTRON OPTICS
19
ELECTRON
SOURCE
CONDENSOR
LENSES
SAMPLE
OBJECTIVE
LENS
PROJECTOR
LENSES
DETECTORS
SPECIMEN PREPARATION FOR TEM
FIXATION DEHYDRATION PROCESSING SECTIONING STAINING
FIXATION
⇨To prevent any change in the tissue and preserve the
tissue as much as possible to its living condition
⇨To prepare the tissue for the further processing so
that the tissue does not disintegrate or tear
⇨No ideal fixative- depends on the tissue type
⇨Glutaraldehyde + osmium tetroxide.
⇨Average time of fixation is 9 h by 4%
⇨ Glutaraldehyde at room temperature and 1 h for
osmium tetroxide
21
DEHYDRATION
⇨ The sample is treated with the series of graded
alcohol:
⇨ 30% ethyl alcohol-10 min
⇨ 50% ethyl alcohol-10 min
⇨ 70% ethyl alcohol- 10 min
⇨ 90% ethyl alcohol-10 min
⇨ 100% ethyl alcohol-10 min
22
PROCESSING
⇨ The ideal embedding medium should have the following
desirable criteria:
⇨ Easy to cut the section
⇨ Stable in electron beam and withstand higher
temperature (200 s °C) at the time of microscopy
⇨ Easy to procure the medium
⇨ Evenly polymerized
⇨ Presently the following media are used for EM: 1. Epoxy
resin 2. Acrylic media 3. Polyester resin.
23
SECTIONING
⇨Semi thin sections and ultrathin sections are made
using ultrathin microtomy.
⇨Sections should be less than 100 nm thick section
and the optimum thickness is 80 nm.
⇨Glass knives
⇨Diamond knives are used
24
STAINING
⇨ Reynold’s lead citrate solution is used for the
staining.
⇨ Lead rapidly reacts with the atmospheric carbon
dioxide and may form lead carbonate as
precipitate.
⇨ Therefore adequate care should be taken to prevent
such precipitation.
⇨ Alternatively uranyl acetate can be used.
25
ADVANTAGES
⇨ Powerful magnification
⇨ Examine structure, composition, and properties of
specimens in submicron levels.
⇨ Image morphology samples
26
DISADVANTAGES
27
⇨ Size, cost, maintenance, researcher training, artefacts.
⇨ Cannot take color pictures.
⇨ Cannot image through thick samples.
⇨ Cannot image surface information.
“
28
Diagnosis TEM+LIGHT
MICROSCOPE
Essential research tool-
life sciences& medicine
SEM are limited in
diagnostic wide spread
distribution unlike TEM.
Real space imaging of
nanoparticles
chemical, electronic and
structure of individual
nanocrystals by electron
probe.
Ultra structures of virus,
function of various viral
components.
Association of
genetically altered
proteins - vaccine
production.
Identification of unknown
virus
Bioterrorism and
emerging diseases
surveillance
APPLICATIONS OF TEM
“
29
Thank you
30

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Transmission electron microscope

  • 1. INTRODUCTION TO ELECTRON MICROSCOPY, TRANSMISSION ELECTRON MICROSCOPY IN DETAIL- INCLUDING FIXATION, PROCESSING & SECTIONING OF SPECIMENS FOR TEM STUDY DR. MOUNIKA. S Post graduate student Department of Oral Pathology & Microbiology SRM Dental College, Ramapuram, Chennai, India
  • 2. CONTENTS  APPLICATIONS OF TEM ADVANTAGES & DISADVANTAGES OF TEM  SAMPLE PREPARATION  FIXATION  PROCESSING  SECTIONING  STAINING  INTRODUCTION  COMPONENTS OF ELECTRON MICROSCOPE  TRANSMISSION ELECTRON MICROSCOPY  PRINCIPLES OF TEM  ELECTRON INTERACTION IN TEM INSTRUMENTATION- VACCUM, ELECTRICAL, MICROSCOPE COLUMN& ELECTRON OPTICS 2
  • 3.  Microscope magnifies the image of the object so that we can visualize the smallest particles.  Wavelength in light microscopy is 300-700 nm  During the first part of the twentieth century, the wave like property of the electron was demonstrated, and subsequently this has been utilized in electron microscope (EM).  Max Knoll & Ernest Rusker- DISCOVERED EM INTRODUCTION
  • 4. v According to De Brogle's formula, λ=h/mv v λ is wavelength, h = 6.626 × 10−34 (Planck’s constant), m = mass and v = speed of the electron. v Increase in speed of electron can decrease the wavelength- better resolution. v Wavelength in EM- 0.2 nm. v EM images provide key information on the structural basis of cell function and of cell disease
  • 5. PROPERTIES OF ELECTRON Electrons have shorter wavelength and provide very high-resolution capacity. It is easy to manipulate Electron gives high brightness Electron beam interacts strongly with matter
  • 7. COMPARISON BETWEEN LIGHT AND ELECTRON MICROSCOPES
  • 8.
  • 9. COMPONENTS OF ELECTRON MICROSCOPE 1. Electron source 2. Sample illumination 3. Objective lens 4. Intermediate and projector lenses 5. Detectors Electron Source Electron gun generates the beam of electrons. It consists of a: (a) Tungsten filament (b) Wehnelt cylinder (cathode shield) (c) Anode plate
  • 10.
  • 12. 12 1 3 5 6 4 2 LIGHT FROM LIGHT SOURCE MAGNIFIED IMAGE BY OBJECTIVE LENS BRIGHTELY ILLUMINATED FIELD OF VISION PASSES THROUGH TRANSPARENT OBJECT VIRTUAL IMAGE BY OCCULAR LENS LIGHT MICROSCOPY
  • 13. 13 1 3 5 6 4 2 COUNTERPART OF LIGHT MICROSCOPE 50% INCIDENT ELECTRONS THROUGH ULTRA THIN SECTIONS 2D IMAGES ARE SEEN PASSAGE OF HIGH VELOCITY HOMOGENOUS ELECTRONS EMERGENT BEAM FOCUSSED TO EML TRANSMISSION ELECTRON MICROSCOPY
  • 14.
  • 16. INSTRUMENTATION OF TEM THE VACCUM SYSTEM THE ELECTRICAL SYSTEM MICROSCOPE COLUMN & ELECTRON OPTICS
  • 17. THE VACCUM SYSTEM 17  Electron beam should be inside a vacum chamber for 2 reasons: 1. To prevent gas molecules colliding with electrons 2. Prevents oxidation of tungsten molecules thus, increasing longevity  A series of pumps are employed it includes, MECHANICAL ROTARY PUMP 1x10- 2Pa DIFFUSION PUMP 1X10 - 5Pa TURBO MOLECULAR PUMP ION PUMP 1x10- 7Pa
  • 18. THE ELECTRICAL SYSTEM 18 HIGH TENSION UNIT LENS CURRENT SUPPLY UNIT VOLTAGE & LENS CURRENT STABILISER UNIT
  • 19. MICROSCOPE COLUMN &ELECTRON OPTICS 19 ELECTRON SOURCE CONDENSOR LENSES SAMPLE OBJECTIVE LENS PROJECTOR LENSES DETECTORS
  • 20. SPECIMEN PREPARATION FOR TEM FIXATION DEHYDRATION PROCESSING SECTIONING STAINING
  • 21. FIXATION ⇨To prevent any change in the tissue and preserve the tissue as much as possible to its living condition ⇨To prepare the tissue for the further processing so that the tissue does not disintegrate or tear ⇨No ideal fixative- depends on the tissue type ⇨Glutaraldehyde + osmium tetroxide. ⇨Average time of fixation is 9 h by 4% ⇨ Glutaraldehyde at room temperature and 1 h for osmium tetroxide 21
  • 22. DEHYDRATION ⇨ The sample is treated with the series of graded alcohol: ⇨ 30% ethyl alcohol-10 min ⇨ 50% ethyl alcohol-10 min ⇨ 70% ethyl alcohol- 10 min ⇨ 90% ethyl alcohol-10 min ⇨ 100% ethyl alcohol-10 min 22
  • 23. PROCESSING ⇨ The ideal embedding medium should have the following desirable criteria: ⇨ Easy to cut the section ⇨ Stable in electron beam and withstand higher temperature (200 s °C) at the time of microscopy ⇨ Easy to procure the medium ⇨ Evenly polymerized ⇨ Presently the following media are used for EM: 1. Epoxy resin 2. Acrylic media 3. Polyester resin. 23
  • 24. SECTIONING ⇨Semi thin sections and ultrathin sections are made using ultrathin microtomy. ⇨Sections should be less than 100 nm thick section and the optimum thickness is 80 nm. ⇨Glass knives ⇨Diamond knives are used 24
  • 25. STAINING ⇨ Reynold’s lead citrate solution is used for the staining. ⇨ Lead rapidly reacts with the atmospheric carbon dioxide and may form lead carbonate as precipitate. ⇨ Therefore adequate care should be taken to prevent such precipitation. ⇨ Alternatively uranyl acetate can be used. 25
  • 26. ADVANTAGES ⇨ Powerful magnification ⇨ Examine structure, composition, and properties of specimens in submicron levels. ⇨ Image morphology samples 26
  • 27. DISADVANTAGES 27 ⇨ Size, cost, maintenance, researcher training, artefacts. ⇨ Cannot take color pictures. ⇨ Cannot image through thick samples. ⇨ Cannot image surface information.
  • 28. “ 28 Diagnosis TEM+LIGHT MICROSCOPE Essential research tool- life sciences& medicine SEM are limited in diagnostic wide spread distribution unlike TEM. Real space imaging of nanoparticles chemical, electronic and structure of individual nanocrystals by electron probe. Ultra structures of virus, function of various viral components. Association of genetically altered proteins - vaccine production. Identification of unknown virus Bioterrorism and emerging diseases surveillance APPLICATIONS OF TEM