2189341 material characterisation · 2020. 8. 15. · history of light (or optical) microscopy...
TRANSCRIPT
Imaging techniques and
optical microscopy
Lecturer: Charusluk Viphavakit, PhD
ISE, Chulalongkorn University
Email: [email protected]: https://charuslukv.wordpress.com
2189341 Material Characterisation
History of light (or optical) microscopy
2189341 Material Characterisation 2https://charuslukv.wordpress.com
❑ Primary means for scientists and engineers to examine the microstructure of materials.
❑ The first microscope was created in ~1590 by two Dutch spectacle-makers, Hans and Zacharias Janssen.
❑ In 1665, Robert Hooke published "Microgphia" which illustrates the objects drawn with the aid of his microscope with the power of 30X.
Eyepiece
Objective
Janssen microscope Hooke microscope
Light or optical microscopy (OM)
2189341 Material Characterisation 3https://charuslukv.wordpress.comhttps://micro.magnet.fsu.edu/primer/anatomy/nikone200cutaway.html
Optical principles
2189341 Material Characterisation 4https://charuslukv.wordpress.com
❑ The optical principles of microscopes include image formation, magnification and resolution.
➢ Image formation can be illustrated by the behavior of a light path in a compound light microscope.
➢ The light path in a microscope goes through an eyepiece instead of projector lens to form a virtual image on the human eye retina.
Eyepiece
Objective
Object
Retina
Primary image
➢ The normal, unaided human eye cannot focus clearly on objects closer than about 250 mm, which is known as the least distance of distinct vision.
➢ The virtual image is often adjusted to be located as the minimum distance of eye focus, which is 250 mm.
Optical principles
2189341 Material Characterisation 5https://charuslukv.wordpress.com
𝑀 = 𝑀1𝑀2 =𝑣1 − 𝑓1 𝑣2 − 𝑓2
𝑓1𝑓2
where 𝑓 is the focal length of the lens.𝑣 is the distance between the image and lens.
➢ The magnification of a microscope can be calculated by linear optics, which tells us the magnification of a convergent lens 𝑀.
Optical principles
2189341 Material Characterisation 6https://charuslukv.wordpress.com
➢ Resolution (𝑅)
▪ The minimum distance between two points at which they can be visibly distinguished as two points.
▪ When the point object is magnified, its image is a central spot (the Airy disk) surrounded by a series of diffraction rings, not a single spot.
Airy disk
▪ Magnification of a light microscope is limited by its resolution.
▪ The resolution of a microscope is theoretically controlled by the diffraction of light.
▪ To distinguish between two such point objects separated by a short distance, the Airy disks should not severely overlap each other.
Optical principles
2189341 Material Characterisation 7https://charuslukv.wordpress.com
➢ Resolution (𝑅)
▪ Controlling the size of the Airy disk is the key to controlling resolution.
𝐼2
𝑑
2
𝐼1 ▪ The size of the Airy disk (𝑑) is related to wavelength of light (𝜆) and half-angle of light coming into the lens (𝛼) .
▪ The resolution of a microscope (𝑅) is defined as the minimum distance between two Airy disks that can be distinguished.
𝑅 =𝑑
2=
0.61𝜆
𝑛 sin 𝛼
where 𝑛 is the refractive index of the medium between the object and objective lens.
Optical principles
2189341 Material Characterisation 8https://charuslukv.wordpress.com
▪ Numerical aperture (𝑁𝐴)
𝑁𝐴 = 𝑛 sin 𝛼 where 𝑁𝐴 is the numerical aperture of the lens.
Object
Objective lens
Aperture
𝛼
• A dimensionless number that characterizes the range of angles over which the system can accept or emit light.
Optical principles
2189341 Material Characterisation 9https://charuslukv.wordpress.com
To achieve high resolution system, what should we do?
𝑅 =0.61𝜆
𝑁𝐴
➢ Resolution (𝑅)
Optical principles
2189341 Material Characterisation 10https://charuslukv.wordpress.com
𝐵𝑟𝑖𝑔ℎ𝑡𝑛𝑒𝑠𝑠 =𝑁𝐴 2
𝑀2
▪ Brightness
• For a microscale object, high magnification is not sufficient.• A microscope should also generate sufficient brightness and contrast of light from the object.
• Brightness refers to the intensity of light.
Transmitted OM:
𝐵𝑟𝑖𝑔ℎ𝑡𝑛𝑒𝑠𝑠 =𝑁𝐴 4
𝑀2Reflected OM:
• The brightness decreases rapidly with increasing magnification.• Controlling 𝑁𝐴 is not only important for resolution but also for brightness.
Optical principles
2189341 Material Characterisation 11https://charuslukv.wordpress.com
𝐶𝑜𝑛𝑡𝑟𝑎𝑠𝑡 =𝐼𝑜𝑏𝑗𝑒𝑐𝑡 − 𝐼𝑏𝑎𝑐𝑘𝑔𝑟𝑜𝑢𝑛𝑑
𝐼𝑏𝑎𝑐𝑘𝑔𝑟𝑜𝑢𝑛𝑑
▪ Contrast
• The relative change in light intensity (𝐼) between an object and its background.
• Visibility requires that the contrast of an object exceeds a critical value called the contrast threshold.
• The contrast threshold of an object is not constant for all images but varies with image brightness.
In bright light, the threshold can be as low as about 3% while in dim light the threshold is greater than 200%.
Optical principles
2189341 Material Characterisation 12https://charuslukv.wordpress.com
➢ Depth of Field (𝐷𝑂𝐹)
▪ The range of position for an object in which image sharpness does not change.
Aperture
Focal plane
𝛼
𝐴
𝐷𝑂𝐹
𝑑
▪ An object image is only accurately in focus when the object lies in a plane within a certain distance from the objective lens.
𝐷𝑂𝐹 =𝑑
tan𝛼=
2𝑅
tan𝛼=
1.22𝜆
𝑛 sin 𝛼 tan𝛼
▪ A larger DOF means a larger 𝑅 and worse resolution.
▪ For a light microscope, 𝛼 = 45◦ and the depth of field is about the same as its resolution.
Instrumentation
2189341 Material Characterisation 13https://charuslukv.wordpress.com
❑ A light microscope includes the following main components;
✓ Illumination system✓Objective lens✓ Eyepiece✓Photomicrographic system✓ Specimen stage
❑ There are 2 types of optical microscope including;
➢ Reflected optical microscope➢ Transmitted optical microscope
The main difference between transmitted and reflected OM is the illumination system.
Reflected vs Transmitted OM
2189341 Material Characterisation 14https://charuslukv.wordpress.com
Silicon wafer
Quartz wafer
Integrated circuits
Ceramics
PMMA
Printed paper documents
Tissues
Cell walls
Crystalline components
Au thin films (100 nm thick)
Instrumentation
2189341 Material Characterisation 15https://charuslukv.wordpress.com
➢ Illumination system
▪ The illumination system of a microscope provides visible light by which the specimen is observed.
▪ There are three main types of electric lamps used in light microscopes;✓ Low-voltage tungsten filament bulb→ Provide continuous spectrum✓ Tungsten–halogen bulbs → Provide continuous spectrum but brighter.
The high filament temperature generates heat so the heat filter is required✓ Gas discharge tubes → Pressurised mercury or xenon vapor providing
extremely high brightness. Discontinuous spectrum for mercury (more common). Cooling system is required.
Instrumentation
2189341 Material Characterisation 16https://charuslukv.wordpress.com
➢ Illumination system
✓ Light lamp✓Collector lens✓Condenser lens✓Objective lens✓Ocular lens (Eyepiece)
Retina
Eye lens
Lamp
Specimen
Illumination system of a transmission OM
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
2189341 Material Characterisation 17https://charuslukv.wordpress.com
➢ Illumination system
Illumination system of a reflected OM
Beam splitter
Relay lens
Lamp
Specimen
Instrumentation
✓ Light lamp✓Collector lens✓Condenser lens✓Objective lens✓Ocular lens (Eyepiece)
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Instrumentation
2189341 Material Characterisation 18https://charuslukv.wordpress.com
➢ Objective lens
▪ The objective lens is the most important optical component of a light microscope.
▪ The magnification of the objective lens determines the total magnification of the microscope because eyepieces commonly have a fixed magnification of 10x, and its resolution determines the final resolution of the image.
▪ The numerical aperture (𝑁𝐴) of the objective lens varies from 0.16 to 1.40.
▪ A lens with a high magnification has a higher 𝑁𝐴.
▪ The highest 𝑁𝐴 for a dry lens (the medium between the lens and specimen is air) is about 0.95. → 𝛼 can be calculated!!!
Instrumentation
2189341 Material Characterisation 19https://charuslukv.wordpress.com
➢ Objective lens
Colour-coded ring for magnification
Objective working parameter/Coverslip thickness (mm)
Specialised optical properties
Magnification 1x 4x/5x 10x16x/20x/25x/32x
40x 60x 100x
Colour-code
Specimen preparation
2189341 Material Characterisation 20https://charuslukv.wordpress.com
➢ The microstructure of a material can only be viewed in a light microscope after a specimen has been properly prepared by sectioning, mounting, grinding, polishing and etching.
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Specimen preparation
2189341 Material Characterisation 21https://charuslukv.wordpress.com
▪ Sectioning
• Generating cross section• Reducing the size• Cutting
• Specimens are too small• Specimens are oddly shaped to be handle• The edge of a specimen needs to be
examined in transverse section• Embedding specimens in mounting
materials (thermosetting polymers)
▪ Mounting
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Specimen preparation
2189341 Material Characterisation 22https://charuslukv.wordpress.com
▪ Grinding/Polishing
• Flattening the surface to be examined• Removing any damage caused by sectioning• Abrading with a graded sequence of abrasives (e.g. SiC), starting with a coarse grit
240 grit 320 grit 400 grit 600 grit
Polishing
RinsingRinsing RinsingGrinding direction
• Polishing is the last step in producing a flat, scratch-free surface.• Abrasives for polishing are usually diamond paste, alumina.• Coarse polishing uses abrasives with a grit size in the range from 3 to 30 μm.
The abrasive size for fine polishing is usually less than 1μm.
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Specimen preparation
2189341 Material Characterisation 23https://charuslukv.wordpress.com
▪ Grinding/Polishing
Effects of grinding and polishing a specimen surface
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Specimen preparation
2189341 Material Characterisation 24https://charuslukv.wordpress.com
▪ Etching
• Generating contrast between microstructural features in specimen surfaces.• A controlled corrosion process by electrolytic action between surface areas with
differences in electrochemical potential.• During etching, chemicals (etchants) selectively dissolve areas of the specimen
surface.
Material Etchant Procedure
Al and alloys 2.5 ml HNO3, 1.5 ml HCl, 1.0 ml HF, 95 ml water Immerse 10–20 s
Fe and steels 1–10 ml HNO3, in 90–99 ml methanol Immerse few seconds to 1 minute
Ti and alloys 10 ml HF, 5 ml HNO3, 85 ml water Swab 3–20 seconds
Al2O3 15 ml water, 85 ml H3PO4 Boil 1–5 minutes
Imaging Method
2189341 Material Characterisation 25https://charuslukv.wordpress.com
➢ The differences in properties of the light waves reflected from microscopic objects enable us to observe these objects by light microscopy.
➢ The light wave changes in either amplitude or phase when it interacts with an object.
Reference wave
Amplitude object
Phase object
➢ The eye can only appreciate amplitude and wavelength differences in light waves, not their phase difference.
Imaging Method
2189341 Material Characterisation 26https://charuslukv.wordpress.com
➢ Bright-Field and Dark-Field Imaging
▪ It is based on contrast due to differences in wave amplitudes.
James A. Sullivan, www.cellsalive.com
Aperture
Shaded areas indicate where the light is blocked.
Bright-field The specimen is evenly illuminated by a light source.
Dark-field The specimen is illuminated by oblique light rays.
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Imaging Method
2189341 Material Characterisation 27https://charuslukv.wordpress.com
▪ Bright-field imaging is the predominant mode for examining microstructure.
▪ Dark-field imaging is used to obtain an image with higher contrast than in bright-field.
James A. Sullivan, www.cellsalive.com
Imaging Method
2189341 Material Characterisation 28https://charuslukv.wordpress.com
➢ Phase contrast microscopy
▪ A useful technique for specimens such as polymers that have little inherent contrast in the bright-field mode.
▪ A phase change due to light diffraction by an object is converted to an amplitude change
▪ The conversion is based on interference phenomenon of light waves.
Phase object
Am
plit
ud
e Constructive interference
Destructive interference
Imaging Method
2189341 Material Characterisation 29https://charuslukv.wordpress.com
➢ Phase contrast microscopy
▪ A condenser annulus, an opaque black plate with a transparent ring, is placed in the front focal plane of the condenser lens.
Image plane
Diffracted light
Non diffracted light
Phase plate
Objective
Condenser
Condenser annulas
▪ The phase plate is placed at the back focal plane of the objective lens. It is a plate of glass with an etched ring of reduced thickness.
▪ The ring with reduced thickness in the phase plate enables the waves of the straight-through beam to be advanced by Τ𝜆 4.
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Imaging Method
2189341 Material Characterisation 30https://charuslukv.wordpress.comGregor T. Overney, California, USA and James A. Sullivan, www.cellsalive.com
Imaging Method
2189341 Material Characterisation 31https://charuslukv.wordpress.com
➢ Polarised light microscopy
▪ It is used to examine specimens exhibiting optical anisotropy.▪ Optical anisotropy arises when materials transmit or reflect light with different
velocities in different directions.
▪ Light, as an electromagnetic wave, vibrates in all directions perpendicular to the direction of propagation. If light waves pass through a polarizing filter, called a polarizer, the transmitted wave will vibrate in a single plane.
Random incident light
Polarised transmitted light
Polarizer
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Imaging Method
2189341 Material Characterisation 32https://charuslukv.wordpress.com
➢ Polarised light microscopy
▪ For a transparent crystal, the optical anisotropy is called double refraction, or birefringence, because refractive indices are different in two perpendicular directions of the crystal.
▪ When a polarized light ray hits a birefringent crystal, the light ray is split into two polarized light waves (ordinary wave and extraordinary wave) vibrating in two planes perpendicular to each other.
Birefringent crystal
High 𝑛 directionLow 𝑛 direction
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Imaging Method
2189341 Material Characterisation 33https://charuslukv.wordpress.com
➢ Polarised light microscopy
▪ As there are two refractive indices, the two split light rays travel at different velocities, and thus exhibit phase difference.
Birefringent object
Ordinary Wave
Extraordinary Wave
Phase difference
Imaging Method
2189341 Material Characterisation 34https://charuslukv.wordpress.comRafat, Cedric, et al. "A crystal-clear diagnosis: acute kidney injury in a patient with suspected meningoencephalitis." Kidney international 86.5 (2014): 1065-1066.Nguyen, Dustin M., et al. "An automated algorithm to quantify collagen distribution in aortic wall." Journal of Histochemistry & Cytochemistry 67.4 (2019): 267-274.
Imaging Method
2189341 Material Characterisation 35https://charuslukv.wordpress.com
➢ Fluorescence microscopy
▪ It is useful for examining objects that emit fluorescent light.▪ Fluorescence is an optical phenomenon; it occurs when an object emits light of a
given wavelength when excited by incident light.
▪ The incident light must have sufficient energy, that is, a shorter wavelength than that light emitting from the object, to excite fluorescence.
▪ It is widely used for polymeric and biological samples which can be stained with fluorescent dyes called fluorescent labeling.
Imaging Method
2189341 Material Characterisation 36https://charuslukv.wordpress.com
➢ Fluorescence microscopy
▪ Reflected light microscope is more commonly used because it entails less loss of excited fluorescence than transmitted light.
▪ A high pressure mercury or xenon light can be used for generating high intensity, short wavelength light.
▪ The light source should be ultraviolet, violet or blue, depending on the types of fluorochromes used in the specimen. Object
Objective
Filter cube
Dichronic mirror
Barrier or emission filter
Exciter filter
Light source
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Imaging Method
2189341 Material Characterisation 37https://charuslukv.wordpress.comhttp://zeiss-campus.magnet.fsu.edu/articles/livecellimaging/images/techniquesfigure5.jpg
Bright-field Fluorescencemicroscopy
Fluorescence technique in live-cell imaging
Confocal microscopy
2189341 Material Characterisation 38https://charuslukv.wordpress.com
➢ A related new technique that provides three-dimensional (3D) optical resolution.
➢ A modern confocal microscope has two distinctive features in its structure: a laser light source and a scanning device. Thus, it is often referred to as the confocal laser scanning microscope (CLSM).✓ The laser light provides a high-intensity beam to generate image signals from
individual microscopic spots in the specimen. ✓ The scanning device moves the beam in a rectangular area of specimen to
construct a 3D image on a computer.
➢ Its major applications are in biology, confocal microscopy can also be used for examining the surface topography and internal structure of semi-transparent materials.
Confocal microscopy
2189341 Material Characterisation 39https://charuslukv.wordpress.com
➢ Working principles:
▪ The laser beam is focused as an intense spot on a certain focal plane of the specimen by a condenser lens, which is also serves as an objective lens to collect the reflected beam.
Laser point source
Detector
Pinhole aperture
Objective lens
Focal plane Specimen
Dichronic mirror
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Confocal microscopy
2189341 Material Characterisation 40https://charuslukv.wordpress.com
➢ Working principles:
▪ The reflected beam from the focal plane in a specimen becomes a focused point at the confocal plane.
▪ A pinhole aperture blocks the reflected light from the out-of-focal plane from entering the detector.
▪ Only the light signal from the focal point in the specimen are recorded each time.
Laser point source
Detector
Pinhole aperture
Objective lens
Focal plane Specimen
Dichronic mirror
Leng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Confocal microscopy
2189341 Material Characterisation 41https://charuslukv.wordpress.com
➢ Working principles:
▪ To acquire an image of the focal plane, the plane has to be scanned in its two lateral directions (x–y directions).
▪ To acquire a 3D image of a specimen, the plane images at different vertical positions should also be recorded.
▪ A scanning device moves the focal laser spot in the x–y directions on the plane in a regular pattern called a raster. After finishing one scanning plane, the focal spot is moved in the vertical direction to scan a next parallel plane.
Image 1,1
Image 1,2
Image 1,3
Image 1,4
x
y
…
z
Scanning direction
Confocal microscopy
2189341 Material Characterisation 42https://charuslukv.wordpress.com
➢ Working principles:
▪ To acquire an image of the focal plane, the plane has to be scanned in its two lateral directions (x–y directions).
▪ To acquire a 3D image of a specimen, the plane images at different vertical positions should also be recorded.
▪ A scanning device moves the focal laser spot in the x–y directions on the plane in a regular pattern called a raster. After finishing one scanning plane, the focal spot is moved in the vertical direction to scan a next parallel plane.
Image 2,1
Image 2,2
Image 2,3
Image 2,4
x
y
…
z
Scanning direction
Confocal microscopy
2189341 Material Characterisation 43https://charuslukv.wordpress.com
Image 2,1 Image 2,2 Image 2,3 Image 2,4
…
Image 1,1 Image 1,2 Image 1,3 Image 1,4
…Image 4,1 Image 4,2 Image 4,3 Image 4,4
Image 3,1 Image 3,2 Image 3,3 Image 3,4
……
…
…
…
…
Software
Confocal microscopy
2189341 Material Characterisation 44https://charuslukv.wordpress.com
➢ Three-Dimensional (3D) images:
▪ The technique of confocal microscopy can be considered as optical sectioning.
▪ A 3D image is obtained by reconstructing a deck of plane images.
Optical sectioning
z
Confocal microscopy
2189341 Material Characterisation 45https://charuslukv.wordpress.comLeng, Yang. Materials characterization: introduction to microscopic and spectroscopic methods. John Wiley & Sons, 2009.
Confocal microscopy
2189341 Material Characterisation 46https://charuslukv.wordpress.com
Pros Cons
Optical sectioning ability Expensive
3D reconstruction Complex to operate
Excellent resolution (0.1-0.2 μm) Chemical labeling
Specific wavelengths of light used High intensity laser light
Very high sensitivity
Imaging Method
2189341 Material Characterisation 47https://charuslukv.wordpress.comhttps://www.olympus-lifescience.com/en/microscope-resource/primer/techniques/confocal/confocalintro/
Confocal microscopy
Fluorescence microscopy