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Simple Microscope • Objective magnification Working Distance • Eyepiece magnification http://micro.magnet.fsu.edu/
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Simple Microscope Objective magnification Working Distance Eyepiece magnification

Dec 21, 2015

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Page 1: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Simple Microscope

• Objective magnification• Working Distance• Eyepiece magnification

http://micro.magnet.fsu.edu/

Page 2: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Illumination (Bright Field)• Simple mirror (historical microscope)• Critical illumination• Koehler Illumination

Summary the field of view should be (reasonably) evenly illuminated the illuminating train should be able to fully illuminate the aperture of an objective of NA = 1.0 the light source should be focused in the object in critical illumination, the light bulb is the light source in Köhler illumination, the light source is an iris diaphragm attached to the illuminator (the field stop) the condenser iris is adjusted for each objective

Page 3: Simple Microscope Objective magnification Working Distance Eyepiece magnification
Page 4: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Staining• Staining is a biochemical technique of

adding a class-specific (DNA, proteins, lipids, carbohydrates) dye to a substrate to qualify or quantify the presence of a specific compound.

• Stains and dyes are frequently used in biology and medicine to highlight structures in biological tissues for viewing, often with the

aid of different microscopes.

Page 5: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Dark Field microscopy

bright Dark

Poor-man`s dark field

Page 6: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Dark Field

Page 7: Simple Microscope Objective magnification Working Distance Eyepiece magnification

DIC (Differential Interference Contrast)Wollaston Prism

Optical Path Length (OPL) = n • t

OPL difference = 2*pi*delta/lambda

delta=(n2 - n1) • t

`Nomarski`

Page 8: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Phase Contrast• Converts phase change to Amplitude change

http://micro.magnet.fsu.edu/primer/techniques/phasecontrast/phaseindex.html

Page 9: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Phase Contrast

Page 10: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Phase Contrast• Converts phase change to Amplitude change

Page 11: Simple Microscope Objective magnification Working Distance Eyepiece magnification

• Converts phase change to Amplitude change

φ(x,y) < < 1

PSF(kx,ky) is the Point spread function (PSF)

Without PC optics

With PC optics

Page 12: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Furhter Contrast Enhancement in Phase Contrast Microscopy

• Select part of illumination

Reduce the size of the fat arrow

Page 13: Simple Microscope Objective magnification Working Distance Eyepiece magnification

Proper Choice of the phase shift reverses contrast