chapter 3 Flashcards

1
Q

magnification

A

ability to enlarge object
-work on microscope because of visible light waves that interact between the curvature of the lens
-image formed by objective lens

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2
Q

resolving power

A

ability to show detail

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3
Q

where is the real image projected on microscope?

A

on ocular where it is magnified again to from the image

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4
Q

total mag equation

A

objective power x ocular power

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5
Q

below 400 nm

A

ultraviolet light

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6
Q

above 700 nm

A

infarred light

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7
Q

average white light nm

A

550 nm

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8
Q

resolving power equation

A

wavelength of light nm divided by 2 (numerical aperture of objective lens)

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9
Q

is a smaller resolving power better?

A

-yes because you see smaller things better
-it is the ability to distinguish two adjacent objects

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10
Q

numerical aperture

A

property of the objective lens

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11
Q

what views smaller than .2 micron/nm

A

electron microscope

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12
Q

light microscope limit

A

200/ .2 micron

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13
Q

why is 200 the limit of microscope

A

because it is all the human eye can handle, visible light limit

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14
Q

numerical apeture

A

set value of each lens and defines the amount of light that is able to be captured

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15
Q

oil immersion does?

A

the oil captures the larger cone of light when using 100x
-oil has refractive properties as the glass, so more light is able to be captures

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16
Q

what happens without oil?

A

light refracts out of lens

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17
Q

bright field

A

specimen is darker than surrounding field
-live or preserved samples
-white light

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18
Q

dark field

A

dark surrounding, bright specimen
-live or unstained specimens
-there is a ring of light that interacts with the sample and bends the light/ illuminates the sample (coin on regular scope)

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19
Q

florescence scope

A

-with UV radiation source and filter
-uses dyes/ florescent molecules that emit visible light when bombarded with shorter UV rays
-can use to diagnose based on what colors light up
ex: antibodies with florescent properties bind to microbe

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20
Q

scanning confocal

A

3d like image
-laser beam of light to scan specimen surface

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21
Q

can the electron microscope samples be alive?

A

no

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22
Q

em types

A

-scanning (color)
-trans (BW)

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23
Q

em

A

-beam of electrons in wavelike patterns interact with sample
-waves are 100,000 times shorter than visible light
-5,000 to 1 mil x
-no objective lens it is a magnet that directs the electrons

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24
Q

trans em

A

through specimen
-darker areas are thicker/ denser parts
-specimen is in think slices
-shoot negative electrons through sample
-BW

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25
Q

why are there dark areas of trans em?

A

because they are thicker areas that are electron dense so they reflect the electrons being shot at them because electrons are neg and they repel each other

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26
Q

scanning em does what

A

detects the electrons that bounce off the specimen so it gets an image of the outside surface
-it is a metal coated specimen
-color

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27
Q

wet mounts

A

-live cells, examine size, motility, shape and arrangement

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28
Q

fixed mounts

A

-dry and heat specimen (heat fixing)
-smear is stained using dyes to permit visualization of cells or cell parts

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29
Q

positive staining

A

the microbes are negatively charged at the surface and attract basic dye
-opposites attract

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30
Q

what charge does basic dye have

A

positive

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31
Q

neg stain

A

microbes will repel the dye and the dye will stain the background (neg dyes/ anionic)

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32
Q

acidic dyes cant?

A

enter the microbe because they are neg and the bacteria is too
-like repel like

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33
Q

simple stain

A

one dye
-size, shape arangement

34
Q

differential

A

primary stain and a counterstain to see cell types or parts
-gram stain, acid fast, endospore

35
Q

endospore stain

A

-differentiates endospores from not endospores

36
Q

structural stain

A

-reveal cell parts that you wouldn’t be able to see ex: capsular or flagellar stain
-ex: in capsule the sugar does not take the stain

37
Q

can gram staining diagnose?

A

it helps eliminate 50% of possibilities either gram (+) or neg
-bacteria differentiated based on cell wall morphology

38
Q

gram +

A

thick peptidoglycan

39
Q

gram -

A

thin peptidoglycan and 2 membranes

40
Q

gram + primary

A

crystal violet will clump/ mordant from iodine after rinse the color is there
-color is trapped in thick polyglycan layer
-crystal violet is positive and will enter the cell and get trapped when it is thick
-decolorizer removes it from the thin ones

41
Q

saffronin

A

negative so it enters all the cells but only stains the ones that are gram negative because purple is the dom color

42
Q

gram - is what color

A

-pink from safronin bc purple washed away bc cell wall too thick

43
Q

how does endospore staining work?

A

the sample needs to be boiled for the stain to work bc they are heat resistant
-green first and it is dom over saffron

44
Q

acid fast is for bacteria with?

A

mycolic acids (lipids)
-it creates the waxy cell wall
-TB bacteria is acid fast
-wax is drug resistant
-bright red

45
Q

what makes TB drug resistant

A

mycolic acids

46
Q

Kirby Bower assay

A

plate coated in bacteria

47
Q

inoculation

A

introduce sample into a container of media to make a culture of growth

48
Q

isolation

A

separate your colony from the growth (one species)
-streak
-pour plate
-spread plate

49
Q

streak plate

A

what we did on agar, flaming loops

50
Q

pour plate

A

3 liquids each with lower dilutions of bacteria poured into plates and as agar solidifies bacteria will grow

51
Q

spread plate

A

diluted bacteria in a liquid sample spread on plate with hockey stick tool

52
Q

single species growing

A

-pure culture
-mult. = mixed culture

53
Q

other colors visible

A

-contaminant

54
Q

16 s gene can?

A

identify microbes
-is the sequence gene

55
Q

gene sequence on microbe

A

can show what they are resistant too

56
Q

media properties

A

-physical state (liquid, semisolid, solid)
-chemical composittion (synth or complex)
-functional type (general purpose, transport, assay etc)

57
Q

semisolid

A

has a solidifying solid agent in low amounts
-measures motility of microbes
-soft agar

58
Q

solid

A

-surface for colony formation
-solidifying agent= agar
-powder heated in liquid then solidifies when cool

59
Q

why do we use agar not jello?

A

jello is collagen based and comes form animals so bacteria would eat it and the agar would have holes
-agar is cellulose/ seaweed based so only marine bacteria might eat it

60
Q

temp agros solids

A

42 celsius

61
Q

temp agar liquid

A

powder melts at 100 celsius

62
Q

synthetic media

A

-know exactly what in it/ formula
-pure organic and inorganic compounds

63
Q

complex/ nonsynth

A

-not chemically definable
-brownie batter mix
-ex: we only know tsa and tsb is soy based

64
Q

what enzyme digests protein in agar

A

tripsin

65
Q

general purpose media

A

-typically non synth.
-grows lots of types of bacteria

66
Q

enriched media

A

blood, serum, etc
-special growth factors for fastidious microbes
-often the microbes that live in people

67
Q

blood agar

A

-strep throat or flesh eating disease (same bacteria)
-for microbes that destroy red blood cells
-clear areas shows circular zone clearing of cells

68
Q

beta hemolysis

A

where bacteria have cleared red blood cells

69
Q

chocolate agar

A

-bubonic plague
-killed blood cells that become brown when the hemoglobin/ iron is exposed to air

70
Q

what media is used for isolation

A

selective because it has stuff that inhibits growth of some microbes ex: antibiotic in a plate when looking for antibiotic resistant microbes
-or salt

71
Q

what makes microbes turn different color

A

differential media
-allows color differences

72
Q

what does bile salt inhibit

A

-gram positive bacteria

73
Q

what causes color change in plate

A

-microbe fermenting sugar producing acid and the H ions released cause a ph change which changes the color of the agar

74
Q

selective and differential

A

mannitol salt agar that lets staph grow bc it likes salt and other microbes wont grow in salt
-as the salt is fermented the ph/ color changes

75
Q

macconkey agar

A

-only gram negative will grow on this plate
-microbe has to eat lactose
-crystal violet and bile salt wont let gram positive grow

76
Q

why does oxygen need to be in water?

A

oxy does not diffuse into water well so there would be less oxygen deeper in the water over time and life would die

77
Q

what reduces oxygen in water?

A

boiling water

78
Q

reducing medium

A

substance that absorbs oxygen so we can see how anaerobic baceria grow
-will grow in its optimal environment (tell based on area of water ex: at top the bacteria want the oxygen)

79
Q

carbohydrate fermentation medium

A

-phenol red broth
-has sugar that can be fermented which changes the ph
-has upside down durum tube

80
Q
A