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Biology > 2.1Microscopy (CP1-practical) > Flashcards

2.1Microscopy (CP1-practical) Flashcards

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1
Q

Why do samples need to be stained for microscopy?

A

Stain binds to structures
Heavy metals- electron microscopes
Coloured dye- optical microscopes
Facilitates absorption of electrons/ wavelengths of light to produce image

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2
Q

Define magnification and resolution

A

Magnification- factor by which the image is larger than the actual specimen

Resolution- smallest separation distance at which 2 separate structures can be distinguished from one another

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3
Q

State the magnification and resolution of a compound optical microscope

A

Magnification x2000
Resolution 200nm

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4
Q

How does an optical microscope work?

A
  1. Lenses focus rays of light and magnify the view of a thin slice of specimen
  2. Different structures absorb different amounts and wavelengths of light
  3. Reflected light is transmitted to the observer via objective lens and eyepiece
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5
Q

What limits the resolution of an optical microscope?

A

Diffraction of light

Any structures closer than half the wavelength of light cannot be distinguished as separate

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6
Q

Describe how transmission electron microscope (TEM) works.

A
  1. Pass a high energy beam of electrons through thin slice of specimen.
  2. More dense structures appear darker since they absorb more electrons.
  3. Focus image onto fluorescent screen or photographic plate using magnetic lenses.
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7
Q

State the magnification and resolution of a TEM

A

magnification: x500 000

Resolution: 0.5nm

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8
Q

Describe how a scanning electron microscope (SEM) works

A
  1. Focus a beam of electrons onto a specimen’s surface using electromagnetic lenses
  2. Reflected electrons hit a collecting device and are amplified to produce an image on a photographic plate.
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9
Q

State the magnification and resolution of SEM

A

Magnification x500 000
Resolution 3-10 nm

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10
Q

Explain how to use an eyepiece graticule and stage micrometer to measure the size of a structure.

A
  1. Place micrometer on stage to calibrate eyepiece graticule.
  2. Line up scales on graticule and micrometer. Count how many graticule divisions are in 100um on the micrometer.
  3. length of 1 eyepiece division = 100um / number of
    divisions
  4. Use calibrated values to calculate actual length of structures.
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11
Q

State an equation to calculate the actual size of a structure from microscopy.

A

I= A/M

Image size= actual size/ Magnification

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Biology (20 decks)

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