Observing the Microbial Cell

Question 1

What is light microscopy?

Answer 1

LM resolves images of individual bacteria by their absorption of light. Light microscopy is limited by the wavelength of light.

Question 2

What are the types of light microscopy?

Answer 2

(1) Bright field
(2) Dark field
(3) Fluorescence
(4) Phase contrast

Question 3

What is electron microscopy?

Answer 3

EM uses beams of electrons to resolve details several orders of magnitudes smaller than those seen under light microscopy

Question 4

What are the types of electron microscopy?

Answer 4

(1) Scanning electron microscopy
(2) Transmission electron microscopy
(3) Cryo-EM

Question 5

With is atomic force microscopy?

Answer 5

AFM uses intermolecular forces between a probe and an object to map the 3D topography of a cell, or cell parts.

Question 6

How are bacterial cells perceived in bright field microscopy?

Answer 6

As dark silhouettes blocking the passage of light. Hence the speciment is viewed as as a dark object against a light filled field or background.

Question 7

What is the maximum resolution of bright field microscopy?

Answer 7

200 nm or 0.2 micrometers.

Question 8

What is the limit magnification of bright field microscopy?

Answer 8

x1000
So in the case of bright field microscopy, if we have a magnification of more than 1000, we won’t see more details because of the physical limitation of our eye

Question 9

What does bright field microscopy require?

Answer 9

Stains

Question 10

Single lens vs Compound lens

Answer 10

The advantage of compound lens microscopes over single lens is that much higher magnifications can be achieved with two lenses. Also, lenses often have aberrations within the glass, so having multiple lenses can correct aberrations. As you increase the glass curvature, the affects of aberrations increases faster than magnification. Having multiple lenses can multiply their magnification with minimal aberrations (as magnification is multiplicative whilst aberrations are additive).

Question 11

What are the two basic types of preparation used to view specimens with a light microscope?

Answer 11

Wet mounts and fixation

Question 12

Explain the wet mount preparation method

Answer 12

The specimen is placed on the slide in a drop
of liquid. Sometimes the liquid used is simply water, but oftenstains are added to enhance contrast. Once the liquid has been added to the slide, a coverslip is placed on top and the specimen is ready for examination under the microscope.

Question 13

Explain the fixation preparation method

Answer 13

The “fixing” of a sample refers to the process of attaching cells to a slide. Fixation is often achieved either by heating (heat fixing) or chemically treating the specimen. In addition to attaching the specimen to the slide, fixation also kills microorganisms in the specimen, stopping their movement and metabolism while preserving the integrity of their cellular components for observation.

Question 14

How do you heat-fix a sample?

Answer 14

A thin layer of the specimen is spread on the slide (called a smear) and the slide is then briefly heated over a heat source.

Question 15

Are heat or chemical fixatives preferred for tissue speciments?

Answer 15

Chemical

Question 16

What is simple staining?

Answer 16

A simple stain adds a dark color specifically to cells but not to the external medium or surrounding tissue. It does not differentiate between different cell types.

Question 17

What is differential staining?

Answer 17

A differential stain stains one kind of cell but not another.

Question 18

What is an important feature of methylene blue (simple) and gram (differential) staining?

Answer 18

These stains are positively charged, allowing them to bind to the negatively charged surface of bacterial cells.

Question 19

What is the difference between gram negative and gram positive bacteria?

Answer 19

Gram positive bacteria have a thicker cell wall whilst gram negative bacteria have thinner cell walls

Question 20

How many layers do gram negative bacteria have and what are they?

Answer 20

3 Layers:

(1) Cytoplasmic/inner/plasma membrane
(2) Cell wall
(3) Outer membrane

Question 21

Hoe many layers do gram positive bacteria have and what are they?

Answer 21

2 Layers:

(1) cytoplasmic/inner/plasma membrane
(2) The cell wall

Question 22

Why do gram positive bacteria need a thicker more protective cell wall than gram negative bacteria?

Answer 22

Because they have no outer membrane

Question 23

What is the gram staining procedure?

Answer 23

(1) Crystal violet is added to the bacterial cells
(2) Iodine solution is added
(3) A decolorizer such as alcohol is added
(4) A weaker stain such as water-soluble safranin is added to stain the sample red
(5) Bright field microscopy is used

Question 24

Why do we add crystal violet in the gram staining procedure?

Answer 24

It stains the peptidoglycan layer

Question 25

Why do we add iodine solution in the gram staining procedure?

Answer 25

It will form a complex with the crystal violet and this complex is a larger molecule than the original crystal violet stain and is insoluble in water

Question 26

Why do we add a decolorizer in the gram staining procedure?

Answer 26

It will release the loosely bound stain (i.e. the crystal violet/iodine complex bound to the peptidoglycan)

Question 27

What does the weaker stain do in the gram staining procedure?

Answer 27

Because it is lighter than crystal violet, it will not disrupt the purple coloration of gram positive cells but will stain gram negative cells red

Question 28

What are other kinds of differential stains besides gram staining?

Answer 28

• Acid fast
• Spore stain
• Negative stain

Question 29

What is acid fast stain used for?

Answer 29

To identify mycobacterium tuberculosis

Question 30

Why do we need acid fast staining to detect mycobacterium tuberculosis?

Answer 30

Mycobacterium contain large amounts of lipid substances within their cell wall called mycolic acid which resist staining by ordinary methods like gram staining.

Question 31

What is the acid fast staining proecure?

Answer 31

(1) Carbol fuchsin is added and, since it has an affinity for mycolic acid, it will bind to the tuberculosis bacterium and stain it pink
(2) With alcohol and heat, carbol fuchsin is removed from cells that are unprotected by a waxy-lipid layer (i.e., non M. tuberculosis cells)
(3) Methylene blue is added to stain the other cells and the excess stain is rinsed off
so M.tuberculosis is stained pink whilst the other cells are stained blue

Question 32

Why do we need spore staining to detect spores?

Answer 32

Because of their tough protein coats made of keratin, spores are highly resistant to normal staining procedures

Question 33

What is the spore staining procedure?

Answer 33

(1) Staining is done with malachite green
(2) Heat is also involved. When samples are boiled with malachite green, the stain binds specifically to the endospore coat.
(3) Spores are then visualized using bright field microscopy

Question 34

What do we use negative stains for?

Answer 34

Negative staining is mostly used to stain cells thart are too delicate to be heat fixed.

Question 35

How can negative stains be visualized?

Answer 35

With either light microscopy to electron microscopy

Question 36

What is the negative staining procedure for LM?

Answer 36

(1) Nigrosine is used which is a black inked fluid. Nigrosine will readily give up hydrogen ions and become negatively charged.
(2) Since the surface of most bacterial cells are negatively charged, the cell surface will repel the stain
(3) Therefore, the glass of the slide will stain but not the cell
(4) The stain darkens the surrounding medium and reveals transparent components such as the outer capsule of a pathogen

Question 37

How do negative stains appear with bright field microscopy?

Answer 37

The bacteria show up as clear spots against a dark background

Question 38

Why is dark field and phase contrast microscopy useful?

Answer 38

It enables us to visualize structures that are too difficult or impossible to detect under a bright field microscope

Question 39

What is the ideal case in which dark field microscopy should be used?

Answer 39

In the case where samples cannot be stained (i.e. they are too sensitive or too small). It is also useful for observing live samples, as well as motile samples. Even viruses can be detected.

Question 40

What is the main limitation of dark field microscopy?

Answer 40

The low light levels seen in the images. This means that the sample must be very strongly illumintaed to see details, but this can damage the speciment. Any dust can also scatter light so you need a medium that is extremely clear.

Question 41

How do speciment appear in final images that use dark field microscopy?

Answer 41

Microbes are visualized as halos of bright light against a dark background.

Question 42

What is the main property dark field microscopy relies on?

Answer 42

The scattering of light. It uses scattered light to detect objects too small to be resolve dby any light rays. Extremely small microbes and thin structures can be visualized. The shapes of the objects are not resolved.

Question 43

What does detection of scattered light require?

Answer 43

A modified condenser arrangement that excludes all light that is transmitted directly. The spider light stop allows only a hallow cone of light to focus on the object. The incident light converges at the object and then generates an inverted hollow cone radiating outward

Question 44

How does phase contrast microscopy work?

Answer 44

Phase contrast microscopy exploits differences in refractive index between the cytoplasm and the surrounding medium or between different organelles. The waves that pass through the object will be out of phase compared to the waves that do not. The waves that pass through the obejct will also get bent

Question 45

What does phase contrast optics depend on?

Answer 45

The principle of interference between two waves in a pattern of alternative zones of constructive and destructive interference. The slight differences in the refractive index of the various cell components are transformed into difference in the intensity of transmitted light

Question 46

What can be seen with phase contrast microscopy

Answer 46

Live cells with transparent cytoplasm, the organelles of eukaryotes can be obserrved with high contrast. The specimen appears darker than the background.

Question 47

What is fluorescence?

Answer 47

The emission of light by a substance that has absorbed light or other electromagnetic radiation.

Question 48

How does fluorescence microscopy work?

Answer 48

The speciment is illuminated with light of a specific wavelength which is absorbed by the fluorophores, causing them to emit light of longer wavelengths/lower energy. So, the light we see comes from the sample itself. The specimen absorbs light of a defined wavelength and then emits light of higher wavelengths.

Question 49

What happens to the excited electrons?

Answer 49

The electronsof the atoms of the sample get excited to a higher-energy orbital and then, when they come back to the ground state, they release a photon.

Question 50

Which has a longer wavelength: the emitted light or the absorbed light?

Answer 50

The emitted light. The longer wavelength means it has a lower energy as well

Question 51

What are fluorescence molecules typically used for in microscopy?

Answer 51

To reveal specific cells or cell parts. Fluorescence can be observed in live organisms, but you can’t resolve the detailed shape of a protein. So you can detect the presence of a specific protein, but you cannot resolve its detailed shape.

Question 52

What is the difference between light microscopy and fluorescence microscopy?

Answer 52

In fluorescence microscopy, there is a filter after the original light source that absorbs all colors except for one, depending on the microscopy. So the light coming to the sample is monochromatic

Question 53

What kind of cells does DAPI detect?

Answer 53

Only dead cells whose DNA is intact

Question 54

What is a dichroic mirror?

Answer 54

A material that reflects light below a certain wavelength but transmits light above that wavelength

Question 55

How do fluorescence dyes differ from bright-field stains?

Answer 55

Bright field stains will bind to the specimen and stain the entire specimen (ex: acid fast staining, gram staining, spore staining) or will be repelled by the specimen and will stain the glass slide (ex: negative staining). On the other hand, a fluorescent dye will
selectively bind to a particular molecule for which it has a high affinity (ex: FITC conjugated to an Ab that will
bind a protein specific to that Ab) and, after having absorbed light at a certain wavelength, will emit light at a longer wavelength. Moreover, the fluorescent dyes will allow the detection of specific molecules, such as
proteins, due to higher resolution, whereas brightfield
stains only allow visualization of entire cells, not
subcellular structures and proteins.

Question 56

What are the common fluorophores?

Answer 56

(1) FITC
(2) AO
(3) DAPI

Question 57

Fluoresceinisothiocyanate (FITC)

Answer 57

FITC binds to amino acids in protiens. They can be conjugated to antibodies and the antibodies are used as probes

Question 58

Acridine-orange (AO)

Answer 58

AO stains double stranded nucleic acids (DNA) and single stranded nucleic acids (RNA) in different colors

Question 59

DAPI

Answer 59

The aromatic rings of DAPI mimics a base pair, enabling intercalation between DNA base pairs. It binds strongly to the A-T rich regions in DNA. It gives a blue stain when it absorbs UV waves.

Question 60

When do we use dyes with chemical affinities?

Answer 60

To label DNA (like with DAPI) and membranes

Question 61

What are dye-labelled antibodies?

Answer 61

Dyes conjugated to antibodies. Antibodies that specifically bind a cell component and are chemically
linked to a fluorophore molecule. The use of antibodies linked to fluorophores is known an
immunofluorescence.

Question 62

What are dye-labelled DNA probes for hybridization?

Answer 62

Dyes conjugated to DNA to localize specific DNA sequences.

Question 63

What is gene fusion?

Answer 63

The expression of a protein fused with a fluorescent protein (reporter protein like GFP)

Question 64

What is one problem associated with GFP?

Answer 64

Proteins fused to GFP may behave differently to the original, non-fused protein.

Question 65

What is super resolution imaging?

Answer 65

Super resolution imaging can define the position of a fluorescent protein with a tenfold better precision than the resolution limit of light magnification. It uses peak intensity in order to generate the microscopy.

Question 66

What does confocal mean?

Answer 66

Confocal = excitation + emitted light are focused together

Question 67

What kind of sample can laser confocal microscopy be used on?

Answer 67

Thick tissue samples

Question 68

How does laser confocal microscopy work?

Answer 68

Reflected emission rays are focused and pass through a pinhole which eliminates unfocused light. This technique allows for an increased optical resolution and contrast by focusing together both the excitation light (from the fluorescence) and the emitted light. It is an advanced form of fluorescence microscopy that uses laser beams to resolve subcellular details, and even to visualize cells in 3D.

Question 69

What does a microscopic laser light source do?

Answer 69

It scans across the specimen, focusing the light in order to remove background noise.

Question 70

When do we use LCM?

Answer 70

We use LCM to eliminate or reduce background noise and if the specimen is lightsensitive. In fact, too much light can be detrimental to the sample. Therefore, laser confocal microscopy is advantageous, since only what we are looking at will be exposed by light, conserving other parts of the sample

Question 71

What is intra-vital microscopy?

Answer 71

A type of microscopy that allows observing biological processes in live animals at a high resolution and makes distinguishing between individual cells of a tissue possible. This variation of LCM allows us to focus on what we want to see. A type of stain is applied on living cells allowing us to visualize the movement of specific molecules (e.g. proteins)