Chapter 10

Question 1

A) What is Taxonomy? What are the three areas of taxonomy and what do they entail?

Answer 1

classification of organisms.
Nomenclature: system that names organisms
Classification: organizing organisms into similair groups
Iidentification: process of identifying an isolate

Question 2

B) What does the term phylogeny mean?

Answer 2

understanding evolutionary relatedness

Question 3

C) What is a strain?

Answer 3

group of similiar isolates

Question 4

D) What are the eight taxonomic categories? [Table 10.1]

Answer 4

Domain
Kingdom
phylum
class
order(- ales)
 family( -aceae)
Genus
species

Question 5

E) What are the three domains? Who created them and how? [Figure 10.1, Table 10.2]

Answer 5

Archea
Eucarya
Bateria
Carl Woese. He did this by taking the rrna sequences of many organisms and classified them based upon that.

Question 6

F) What was the accepted scheme before the domains were created?

Answer 6

The five kigdom classification
plantae
fungi
anamalia
protista
prokaryota

Question 7

G) What is Bergey’s Manual of Systematic Bacteriology? [Table 10.3]

Answer 7

This is the “bible” this is the guide of classification of different organisms

Question 8

H) How are bacteria given names?

Answer 8

Some were given names in the past due to the founder, but now we use names that explain characteristics of the bacteria and use a latin suffix

Question 9

A) How can you identify microorganisms without sophisticated equipment? [Table 10.4]

Answer 9

phenotypic characteristics
Microscope morphology
stains
biochemical tests

Question 10

B) What are the benefits of doing a wet mount? [Figure 10.2]

Answer 10

You do not denature the bacteria when heat fixing. Especially when trying to get the right size and shape

Question 11

C) What is a Gram stain? How is it used? [Figure 10.3 a]

Answer 11

This is a staining technique that help differntiate between gram neg. and gram pos. cells

Question 12

D) What organisms do you test for with an acid fast stain? [Figure 3.15]

Answer 12

This helps identify mycobaterium especially tb

Question 13

E) What are some examples of clues given by colony morphology?

Answer 13

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Question 14

F) How would a clinical lab use Blood agar and MacConkey agar? [Figure 4.10, Figure 4.11]

Answer 14

Blood agar helps determine via the type of hemolysis wether it is strptococus pyogenesm (strep) produces bata hemolysis or clear zone.
and
streptococcus that is naturally in all throats. Produces alpha hemolysis which produces green
Then MacConkey:
this shows wether there is lactose fermenters ( selective for gram neg rods

Question 15

G) What biochemical test can be used for a more certain identification? What do they find? [Table 10.5, Figure 10.4]

Answer 15

catalase test: detects to see if there is catalase by adding h2o2
Urease: which you add urea to see if if is broken down forming co2 and ammonia making it more alkaline
go over 10.5 on pg 243!!!!!!!!

Question 16

H) Streptococcus pyogenes has what catalase and hemolysis result?

Answer 16

beta hemolysis and catalase neg

Question 17

I) How are pH indicators used in biochemical tests? [Figure 10.6]

Answer 17

they help you know what products are being made, and therefore different enzyme of that cell

Question 18

J) What is a dichotomous key? [Figure 10.5]

Answer 18

A flow chart of tests that either give neg or positive results.

Question 19

K) Can some bacteria have biochemical test without a culture? Give an example.

Answer 19

When testing for h pylori which produces urease. SO you have patient drink urea with a radioactive isotope. if h pylori positive the urea will break down and co2 will be produced and is measure via breathing into a baloon!

Question 20

L) What is the API system? [Figure 10.6]

Answer 20

this is much faster than doing individual medias. This you can take your organism in liquid through a special tube with sections containing different differential media which was previously dried, but then rehydrated.

Question 21

M) What is an Enterotube II? [Figure 10.6]

Answer 21

similiar to api system, but has a metal rod which touches the colony and then you pull the rod through to innoculate the media

Question 22

N) What is the VITEK 2 system?

Answer 22

is a card with wells of differential media that is later read by a computer

Question 23

O) How can you use the proteins and polysaccharides to identify some prokaryotes?

Answer 23

some have special protiens or polysacharides in there external structure. you can detect these using antibodies.

Question 24

P) What is FAME? How is it done?

Answer 24

some differ in fallty acid composition. So they take bacteria and put them in chemicals that tuen them into viatal methyl ester form these are annalyzed using gas chromotography.

Question 25

A) What is a Nucleic Acid Probe? How are they used? [Figure 10.7]

Answer 25

they are used to find a specific nucleotide sequence. So take a single strand piece of dna labeled with a detectable tag. most of these rely on more dna so they will be introduced to colonies, or cause a cell to do preliminary amplification.

Question 26

B) What is FISH? How is 16S ribosomal RNA involved?

Answer 26

this instead of having is bind to dna has it bind to rrna which is large in number in the cell

Question 27

C) What is a signature sequence?

Answer 27

sequence in rrna that characterizes a certain species

Question 28

D) What are NAATs? How are they used?

Answer 28

nucleic acid amplification tests: they are used to up production of specific segents of dna. This is used to help detect organisms in small numbers

Question 29

E) Why is rRNA useful in microbial identification? [Figure 10.8]

Answer 29

their sequences are stable and do not work under much mutations. The also hare many in number

Question 30

F) What makes the 16S rRNA so special?

Answer 30

it is moderate in size

Question 31

G) How can you detect and identify a microbe that cannot yet be cultured such as Tropheryma whipplei?

Answer 31

using rdna you replicate it many times making it possible to detect

Question 32

A) When can distinguishing different strains of a microbial species be especially useful? How is it done? [Table 10.6]

Answer 32

This can help them find the source… or where the illness came from because there are many different strains. bio chem typing

Question 33

B) What is a biovar or biotype? Give an example.

Answer 33

The biochemical type i,e, cholera has a specific one that is a way you can trace it

Question 34

C) How do you distinguish different types of E. coli? [Figure 10.9]

Answer 34

by the antigenic type of their flagella

Question 35

D) What are RFLPs? How can you observe them? [Figure 10.10]

Answer 35

restricted length pollymorphism:

compair fragment sizes of dna to others (finger prints)

Question 36

E) What is PulseNet? Who established it and for what reason? [Perspective 10.1]

Answer 36

cdc’s catalog of rflp’s of different strains

Question 37

F) What is MLST?

Answer 37

newer way of gedtting dna ‘s 7 nucleotide sequences and comparing them

Question 38

G) What are bacteriophages? How do you use them to type microorganisms? [Figure 10.11]

Answer 38

using different phages( carriers of forign dna)m if bateria are suseptible they will lyce.

Question 39

H) What are antibiograms? How are they done? [Figure 10.12]

Answer 39

antibiotic tests on a bacteria

Question 40

A) What is an evolutionary chronometer? What do they provide?

Answer 40

peices/ equences of dna that tell a estimated time or when it evovled from another organism

Question 41

B) What is a phylogenetic tree? [Figure 10.13]

Answer 41

like family tree, but of what species evolved from what

Question 42

C) What is horizontal gene transfer?

Answer 42

genes being tranfered from one prokaryote to another organism

Question 43

D) What methods can you use to classify Prokaryotes? [Table 10.7]

Answer 43

pg 251!

Question 44

E) Why and how has 16S rRNA revolutionized the classification of organisms.

Answer 44

because r rna is in all organisms and because it is used often it cannot contain a lot of mutations!

Question 45

F) How can you use DNA hybridization to check relatedness?

Answer 45

take dna of one and see if it will hybridize or anneal to anothers. if 70% does then they are considered the same species.

Question 46

G) How do you use G + C content to see how closely related to organisms are? [Figure 10.15]

Answer 46

if gc content is a sm %tage off they cannot be related

Question 47

H) What is numerical taxonomy?

Answer 47

q