Microscopy

Question 1

What is the use of microscopes?

Answer 1

Microscopes used to view objects/specimens that are not visible to the naked eye.

Invented by eyeglass makers in 1590s

Question 2

What are the characteristic parts of a microscope?

Answer 2

• Light source
• Detector
• Objective
• Specimen
• Light conditioning system

Question 3

Describe the types of detector used in microscopes

Answer 3

Photomultiplier tubes (PMT), CCD

PMTs increase signal and transform it into data read by a computer

Question 4

What is the purpose of the light conditioning system?

Answer 4

Light conditioning system allows light to reach specimen

Question 5

Name different light conditioning systems

Answer 5

• Kӧhler illumination
• Phase ring
• Wollaston prism and polarizers
• Filter cubes (for fluorescence

Question 6

What are the different light sources for microscopes?

Answer 6

Halogen bulb, sunlight, lasers etc.

Question 7

How do we ensure all microscopes work to a standard?

Answer 7

To ensure correct functioning of the objectives and to quantify what we see there needs to be constants in place

Question 8

What is the approximate thickness of a light microscope cover glass?

Answer 8

Cover glass (0.17- 0.18 mm) - anything thicker = objective has to be corrected

Question 9

What are samples embedded in for light microscope use?

Answer 9

Sample surrounded by embedding medium (might contain anti-bleach agent)
on a glass slide

Question 10

What does the box in light microscopes enable?

Answer 10

Allows for life imaging as prevents focus instability

Question 11

What is the effect of temperature on light microscopes?

Answer 11

Small changes in ambient temperature => thermal expansion / contraction in:

• microscope stand
• stage
• objective

> thereby changing the plane of focus

Question 12

How is temperature regulated in light microscopes?

Answer 12

An incubator box combined w/ a precision air heater ensures specimen and microscope temperature remain equilibrated and tightly controlled

Question 13

Describe the light microscope box structure

Answer 13

> Custom design for individual microscopy setup

Intricate system of openings and doors for comfortable access to microscope controls and specimen

Question 14

Describe the structure of the light microscope incubator cube

Answer 14

Highest quality fan, controller cube with external, low vibration and low-nose design

Question 15

What is the role of the light microscope cube?

Answer 15

One side prevents drastic temperature changes and also maintains CO₂ / O₂ levels to keep specimen alive

Question 16

How is the airflow regulated in the light microscope?

Answer 16

A controller allows adjustment of air flow and %CO₂

Possibility of guiding gas stream through bottle of water to diminish loss of humidity

Question 17

How is the live cell culture device enclosed in a light microscope?

Answer 17

Airtight table top encloses the live cell culture device

Question 18

What time considerations are required when deciding what microscope / sample to use?

Answer 18

Need to consider the time required and how to preserve the sample for that long

Question 19

Describe the different experimental timescales of viewing different samples

Answer 19

Development of zebrafish embryo requires hours and even more complex animals may need days

To see how a microtubule extends / shrinks only requires seconds

Question 20

What are the inconveniences of having longer timescales?

Answer 20

In longer timescales:
- Stability 
- Viability 
- Possibility
- Multi-portion timelapse require different complex 
  algorithms

Question 21

What problems need to be overcome when using short experimental timescales?

Answer 21

For shorter timescales:
- Ensure magnifier used has ability to capture imaging
quickly
- Need to distinguish environment from sample
- Artefacts in multichannel / 4D imaging

Question 22

What is the triangle of frustration?

Answer 22

3 factors of microscope use that are compromised between depending on what we need to investigate

Question 23

What are the 3 factors of the triangle of frustration?

Answer 23

• Spatial resolution
• Sensitivity
• Temporal Resolution

Question 24

What is temporal resolution?

Answer 24

How long and how fast images need to be taken

Question 25

What is sensitivity?

Answer 25

The ability to pick up image in lower light conditions (quality of image)

Question 26

What is spatial resolution?

Answer 26

The pixel no.
> bigger cube image taken faster but lower quality low resolution

> smaller cube image taken slower but higher quality high resolution)

Question 27

How does time taken effect image resolution?

Answer 27

To get a high resolution image, microscope requires more time to collect data and CPU to read it

Question 28

How long does it take for a microscope to produce a low resolution image?

Answer 28

Microscope can generate a low resolution image very quickly

Question 29

Why may we sacrifice high resolution when capturing an image?

Answer 29

In fast occurring processes, capturing an image can be hard as everytime you look at the image it will have changed

Need system that captures images fast: Sacrifice resolution to capture image

Question 30

Why are non-living specimens usually captured in higher resolution?

Answer 30

In non-living specimens, there is no time limit so can spend longer on an image and gain higher resolution

Question 31

What is a microscope objective?

Answer 31

An objective is a series of high quality pieces of glass placed in a particular way, allowing us to see magnified images

Question 32

What is the magnification?

Answer 32

The magnification tells us how much bigger the image will be seen compared to original
Can be colour coded or written as number (e.g. 40x)

Question 33

What is an objective application?

Answer 33

Certain objectives are more suitable for certain applications over others - objective will be marked for it’s suitable applications

Question 34

Why may an immersion medium be required?

Answer 34

Immersion medium may be needed (e.g. water, oil) to see specimen - looking through air won’t produce an image and vice versa

Question 35

What is a working distance of an objective?

Answer 35

Distance from sample the objective can work at (e.g. 0.20 mm)

Question 36

What markings are present on an objective?

Answer 36

• Magnification
• Application
• Lens - image distance
• Cover slip thickness (mm)
• Working Distance (mm)
• Numerical aperture
• Immersion medium

Question 37

What is the role of the objective aperture?

Answer 37

The aperture of the objective determines the resolution

Question 38

How can we determine resolution from numerical apertures?

Answer 38

The higher the numerical aperture the better the resolution power of the objective

Question 39

What is the relationship between resolution and magnification?

Answer 39

RESOLUTION ≠ MAGNIFICATION

Question 40

What features allows an image to be seen using a light microscope?

Answer 40

Light and Lenses to illuminate and magnify

Question 41

Describe the fundamental Setup of a light microscope

Answer 41

Always contain:

• Light source
• Trebles
• Rings / Lens to modify light source if needed
• Objective magnifies image
• Viewed through ocular

Question 42

What are the different types of light microscopy techniques?

Answer 42

DIC
Brightfield
Phase Contrast

Question 43

What is brightfield light microscopy?

Answer 43

Brightfield - all light reaches sample

Question 44

What is DIC microscopy?

Answer 44

DIC - condenses light through a smaller area

Allows for 3D

Question 45

Describe phase contrast light microscopy

Answer 45

Phase contrast - uses a phase ring with a small circumference where light can go through.

Question 46

What are the pros of using light microscopy for histology?

Answer 46

Pros: Gain general idea of tissue

Question 47

What is the disadvantage of light microscopy for histology?

Answer 47

Cons: Lacks details, hard to distinguish between cells

Question 48

How is light microscopy used to identify ovulation site in an ovary?

Answer 48

Use chemicals that react with particular parts of tissue based mainly within pH range of sample

Question 49

What enables the chemicals to stick to the different types of tissues?

Answer 49

There are chemicals that have a higher affinity for basic tissues and others have a higher affinity for acidic tissues

Question 50

What is immunohistochemistry?

Answer 50

Protein of interest is found using antibodies produced against an exogenous agent with high affinities for particular antigens

Question 51

What is the use of immunohistochemistry?

Answer 51

allows us to see specific proteins

Question 52

How does phase contrast work?

Answer 52

Reduces the amount of grey’s (black or white) - increasing contrast to see cell margins

Question 53

What is a major use of brightfield?

Answer 53

Colour brightfield used to see life events

e.g. Heart Cell Differentiation
Differentiation of cardiomyocyte-like cells derived from adipocytes.

Question 54

How are samples maintained in colour brightfield microscopy of life imaging?

Answer 54

Need to control and regulate temperature and CO₂ to keep sample alive

Question 55

What are the 2 methods of life imaging ?

Answer 55

1. Take fixed images over a course of time

2. View under microscope and monitor periodically to see development

Question 56

What cell feature is viewed using time-lapse microscopy?

Answer 56

Cell migration also viewed via time-lapse microscopy

> takes images after specific time intervals and collates them together

Question 57

How do (~smallpox) virus infected cells migrate?

Answer 57

When the cells are infected they migrate towards empty area where they extend and send viral particles to one another

Question 58

How did using time-lapse microscopy enable us to prevent viral spread?

Answer 58

Allowed us to remove specific gene from infected cells prevented migration and spread of infection

Question 59

Describe the light source in e- microscopes

Answer 59

The light source in electron microscopy is a beam of electrons and not light

Question 60

Describe transmission electron microscopes

Answer 60

TEM not 3D, beam of e- transmitted through ultra-thin specimen, interacting with specimen as it passes through (Uranyl acetate used as a stain)

Question 61

Describe an EM image

Answer 61

e- can’t pass through denser areas show up darker and lighter areas are less dense

Question 62

How is the image detected in EM?

Answer 62

e- eventually end up at a viewing screen connected to a camera / PMTs to view higher resolution images

Question 63

Describe the use of scanning electron microscopes

Answer 63

sample treated with specific reagents, scans a beam of electrons through sample creates 3D images (key difference with transmission!)

Question 64

How do fluorescence microscopes create fluorescence?

Answer 64

Uses a particular wavelength of light; fluorescence light

Question 65

How do fluorescence microscopes produce an image?

Answer 65

1. Light modified through various filters
2. Specimen exposed to light
3. Specimen absorbs light (excitation) and releases energy
   (emission)
4. Emission is taken up to the oculars

Question 66

How is fluorescent image detected in a fluorescent microscope?

Answer 66

PMTs transform the fluorescent image into computer data that is safe to view

Question 67

What is fluorescence?

Answer 67

Fluorescence is the ability of certain types of molecules to absorb light and generate energy

Question 68

Describe the mechanism of fluorescence

Answer 68

Specimen exposed to light absorbs light (excitation) releases energy (emission)

Question 69

Why is fluorescence a finite feature?

Answer 69

Several rounds of this cycle will eventually lead to energy loss and molecule gets destroyed no fluorescence

Question 70

What is stokes shift?

Answer 70

Difference between wavelength used to excite molecule of interest, and emission wavelength of molecule after energy release

Question 71

Describe the wavelengths of emission and excitation

Answer 71

Excitation < emission wavelength always bigger

Question 72

Why is emission always larger than excitation?

Answer 72

Due to energy loss the emitted light is shifted to longer wavelengths relative to the excitation light

Question 73

Why may photo-bleaching occur?

Answer 73

Bleaching of fluorochrome; due to high intensity illumination
Causes fluorochrome to lose permanently their ability to emit light

Question 74

How can photo-bleaching be prevented?

Answer 74

→Work w/ reduced excitation light intensities or gray
filters
→ Use shorter exposure times / higher gain settings and
longer intervals during time lapse studies
→ Use anti-bleach in mounting media

Question 75

Describe the variety of fluorochromes available currently

Answer 75

Now have lots of fluorochromes able to emit and absorb most wavelengths of light spectrum

Question 76

Give an example of a fluorescent protein

Answer 76

GFP: These proteins are naturally found in light-producing cells of cnidarians

Question 77

How can fluorescent proteins be used for live imaging?

Answer 77

Fluorescent proteins can be fused with other proteins and introduced in cells via transfection

Allows live study of fluorescent tags in living cells / organisms

Question 78

Why are GFP better than antibodies?

Answer 78

Can tag GOI with GFP gene via electroporation; allow slive study of fluorescent tags in living cells

Question 79

When is a confocal fluorescent microscope used?

Answer 79

To view specific portions of a sample a confocal (can be fluorescence) microscope is used.

Question 80

How does a confocal fluorescent microscope setup differ?

Answer 80

The microscope setup is the same, except for a laser light source

Question 81

Outline the mechanism of a confocal fluorescent microscope

Answer 81

1. Laser emits particular wavelength (can have specific
   lasers for different wavelengths)
2. Laser travels through different modifiers to reach
   sample
3. Sample excited due to fluorophores reaching high
   energy
4. When fluorophores lose energy they emit a certain
   wavelength collected by a PMT → CPU → digital image

Question 82

How do wide field and confocal microscopes differ?

Answer 82

The difference between confocal and wide field microscopes is the detector pinhole - metal with a hole in

Question 83

What is the purpose of the detector pinhole in fluorescent microscopes?

Answer 83

Of all light emitted by sample, only the light passing through pinhole will reach PMTs to form image - helps remove background and allows us to see very specific areas of sample

Question 84

Why are confocal images clearer than wide field?

Answer 84

Higher z-resolution and reduced out-of-focus-blur make confocal pictures crisper and clearer

Question 85

Describe the sample size seen by confocal microscopes

Answer 85

Only a small volume can be visualised by confocal microscopes at once

Question 86

What is the limitation of sampling bigger volumes?

Answer 86

Bigger volumes need time consuming sampling and image reassembling