Lecture 4 - Exam 1 Flashcards

Question 1

Q

Describe the growth of a cell.

Answer

A

Increases in mass of the cell

Question 2

Q

Describe the growth of a population.

Answer

A

Increase in number of cells.

Question 3

Q

What are the factors that affect microbial population growth?

Answer

A

Acquisition of nutrients, catabolism of nutrients, anabolism of vital cell compartments, replication of genetic material, division of a cell into two daughter cells and start over.

Question 4

Q

What are the many ways to measure cell population growth?

Answer

A

Turbidity, viable plate counts, total cell counts (microscopic counts), electronic cell counts, membrane filtration, dry weight, protein measurements, most probable number, measures of metabolic activity.

Question 5

Q

Regarding the ways to measure cell population growth, what do we have to do in order to get very precise numbers?

Answer

A

Multiple measurements.

Question 6

Q

When measuring turbidity, what is one of the most widely-used methods to estimate population numbers?

Answer

A

A spectrophotometer.

Question 7

Q

(Turbidity measurement) Within limits, the __________ by a bacterial cell is proportional to ___________.

Answer

A

Within limits, the amount of light scattered by a bacterial cell is proportional to its mass.
So, light scattering is proportional to total mass.

Question 8

Q

(Turbidity measurement) If average mass per cell remains a constant, light scattering can be used to measure _______?

Answer

A

Changes in cell number (i.e. growth).

Question 9

Q

What is actually being measured when using a spectrophotometer in a turbidity measurement?

Answer

A

The fraction of light transmitted through the culture, not the scattered light.

Question 10

Q

In mathematical terms, what does spectrophotometer provide?

Answer

A

The log of the reciprocal of the fraction of transmitted light.

Question 11

Q

What is the Beer-Lambert Law?

Answer

A

States that the absorption of light is directly correlated to the concentration of a solute (or cells, in this case) in a solution.

Question 12

Q

(Turbidity measurement) The fraction of light does what when the density of the culture increases?

Answer

A

Decreases exponentially.

Question 13

Q

Why aren’t OD readings negative?

Answer

A

We actually obtain a negative number, but since we are human and do not like a decreasing, negative number with increasing cell density, we take the reciprocal log to give a positive number.

Question 14

Q

What are the advantages of using a spectrophotometer to measure turbidity to estimate population numbers?

Answer

A

Simple, fast and inexpensive

Question 15

Q

What are the disadvantages of using a spectrophotometer to measure turbidity to estimate population numbers?

Answer

A

Limited linear range, need standard curve of optical density vs cell count, wavelength can be different for different bacteria (normally at OD600)

Question 16

Q

What are the advantages of direct counts?

Answer

A

Accurately measures total number of cells

Question 17

Q

What are the disadvantages of direct counts?

Answer

A

No distinction between live and dead cells (unless live/dead stain used), not accurate for low density cultures, manual, very tedious

Question 18

Q

We don’t usually use the method of direct counts unless we have?

Answer

A

An electronic cell counter (very expensive, but more accurate and can determine cell count and cell size).

Question 19

Q

What is the second most commonly used technique for estimating population growth?

Answer

A

Cultured counts

Question 20

Q

What are the advantages for cultured counts?

Answer

A

Counts only living cells that can form colonies, to determine colony forming units per mL.

Question 21

Q

What are the limitations of using culture counts?

Answer

A

Only gives counts for culturable species, counts only living cells that can form colonies, easy to underestimate the number of cells due to clumping, assumes that every live cell forms a viable colony, need to know appropriate growth conditions (medium, pH, temp), several days to acquire results.

Question 22

Q

The vast majority of bacterial species cannot currently be ________.

Answer

A

Cultured in vivo

Question 23

Q

What is the “Great Plate Count Anomaly?

Answer

A

When every environmental sample has a big difference between the number of cells observed by direct counting compared to the number of colonies counted on a plate. Many factors that can cause this, a few being: choice of growth medium and requirement for nutrition from other microbes.

Question 24

Q

Uncultivated microbial species are “as-yet-uncultured,” NOT ______

Answer

A

Unculturable microbes.
Note: A majority of microbes do not grow on synthetic media.

Question 25

Q

What is a dry weight measurement?

Answer

A

In dry weight methods, cells are harvested, dried, and weighed. It is fairly accurate, takes time, and there is a need to generate a standard curve of cell/weight for given growth condition.

Question 26

Q

What is a protein measurement?

Answer

A

Measure total protein concentration of cell using Bradford colorimetric assay. It takes times, and there is a need to generate a standard curve of total protein concentration/cell for given growth condition.

Question 27

Q

What are the four phases of cell growth?

Answer

A

Lag phase, log phase, stationary phase, and death or decline phases. Each phase can be very different for different prokaryotic species.

Question 28

Q

Do laboratory conditions reflect actual environments in which microorganisms have evolved?

Question 29

Q

What is the lag phase in bacterial cell growth?

Answer

A

There is no increase in number of living bacterial cells. It is a time of adjustment in a new environment.

Question 30

Q

What are the specifics of what goes on in lag phase of bacterial cell growth?

Answer

A

Recovery of cells from toxic metabolites in the previous environment, synthesis of new enzymes or cofactors, many dead cells in the inoculum rather than live cells (causes the lag in the curve), and the size of cells (mass) increases before replication starts.

Question 31

Q

What is the log/exponential phase in bacterial cell growth?

Answer

A

Exponential increase in number of living bacterial cells. Cell mass increases exponentially over time.

Question 32

Q

What are the specifics of what goes on in log phase of bacterial cell growth?

Answer

A

Fastest growing phases due to maximal utilization of available nutrients and optimal environment conditions for cell division, the number of ribosomes in actively growing E. coli cell can be 70,000, and primary metabolites are produced, meaning waste compounds are associated with rapid growth.

Question 33

Q

What are the different variables for exponential/log phase?

Answer

A

G = t/n
G = generation time
t = time per generation
n = number of generations

Question 34

Q

What is generation time?

Answer

A

The rate of exponential growth of a bacterial culture.

Question 35

Q

During exponential growth, what happens to the mass in the culture?

Answer

A

It doubles each generation.

Question 36

Q

How can growth kinetics actually be useful?

Answer

A

When trying to determine starting culture concentration.

Question 37

Q

What is the stationary phase of bacterial cell growth?

Answer

A

Plateau in number of living bacterial cells ; rate of cell division and death roughly equal. When conditions for logarithmic growth have diminished, there is a slowdown and eventual cessation of population growth.

Question 38

Q

What are the specifics for the stationary phase of bacterial cell growth?

Answer

A

Cultures enter stationary phase when:
Essential nutrients have been exhausted, accumulation of toxic waste products, changes in environment that affects the cell (pH fluctuation, depletion of O2 for facultative anaerobes).

Question 39

Q

What is the primary sigma factor for bacteria during stationary phase?

Question 40

Q

What is RpoS (stationary phase)?

Answer

A

Is a master regulatory factor for stationary phase and stress and starvation gene expression.

Question 41

Q

Does metabolism stop in stationary phase?

Answer

A

NO!
Secondary metabolites are produced that help microorganisms compete with on another, like antibiotics.

Question 42

Q

What are the changes associated with stationary phase?

Answer

A

Metabolic activity changes: There is an increased metabolic breakdown and resynthesis of protein and RNA.
Developmental changes: reduction in cell size and metabolic activity, morphological changes (from rod to cocci), changes in surface properties (increased adhesive properties), changes in protein composition.
Spore production: spores are metabolically dormant cell type. This is a differentiated cell type produced in response to stressful environmental stimuli (prolonged starvation, pH fluctuation, osmotic fluctuation, oxidative stress).
Stringent response

Question 43

Q

What is a stringent response?

Answer

A

A temporary inhibition in synthesis of ribosomal RNA (rRNA) and transfer RNA (tRNA).
Occurs when cells are starved for an amino acids. This caused “uncharged” tRNA to accumulate and the uncharged tRNA activated an enzyme called RelA.

Question 44

Q

What does RelA do?

Answer

A

Synthesizes ppGpp (alarmone), which slows transcription of ribosomal RNA, resulting in fewer ribosomes.

Question 45

Q

Cell entering stationary phase also become more resistant to __________.

Answer

A

Environmental stresses, such as high temperature, osmotic stress, and certain chemicals.

Question 46

Q

(Stationary Phase gene expression) Cells entering stationary phase become more resistant to environmental stresses. In Gram negative cells, what are these resistance properties due to?

Answer

A

The synthesis of a starvation sigma factor, RpoS. This master regulator regulates expression of at least 60 genes induced by carbon starvation.

Question 47

Q

RpoS is also a regulator for stress response in _________. Is it tightly controlled/regulated?

Answer

A

Exponentially growing cells.
Yes, tightly controlled/regulated and needs to be turned on and off depending on environmental conditions.

Question 48

Q

(Stationary Phase Gene Regulation: Alarmones)
What does an efficient control of metabolism do?
What are the compounds that can accomplish all this?

Answer

A

Senses stress, adjusts growth accordingly, mandates gene expression, and ultimately provides a fitness advantage over poorly-adapted microbial competitors.
The second messenger molecules (p)ppGpp are compounds that can accomplish all this.
(p)ppGpp are referred to as alarmones.

Question 49

Q

When bacteria experience growth-limiting environmental conditions, the synthesis of alarmones is induced by which enzymes?

Answer

A

RelA and SpoT

Question 50

Q

High levels of (p)ppGpp induce what?

Answer

A

The stringent response.
The stringent response allows bacteria to quickly reprogram transcription in response to changes in nutrient availability.

Question 51

Q

What specifically happens during the stringent response?

Answer

A

Ribosomal RNA and transfer RNA synthesis is downregulated, stress-related genes are upregulated, messenger RNA stability and translation altered (decreases), and allocation of scarce resources optimized.

Question 52

Q

How well is rRNA synthesis understood?
Ribosome synthesis is coupled with what?

Answer

A

Not well.
Coupled to growth rate.

Question 53

Q

Amino acid starvation controls…?

Answer

A

The rate of cell growth, but also inhibits ribosome synthesis.

Question 54

Q

The stringent response is _____-dependent synthesis of ppGpp.

Question 55

Q

What is the SpoT enzyme?

Answer

A

A bifunctional enzyme synthesized in carbon- and energy-limited environments. Synthesizes and degrades ppGpp.

Question 56

Q

What is the death phase of bacterial cell growth?

Answer

A

Exponential decrease in number of living bacterial cells.
Complete depletion of energy occurs -> programmed cell death.

Question 57

Q

What are Viable But Not Culturable (VBNC) bacteria?

Answer

A

Bacteria have reduced metabolic activity and may not grow on nutrient rich media, but may live on less nutrient rich media, as they are adapted to live in less nutrient rich environments.

Question 58

Q

What is the long-term stationary phase?

Answer

A

Mutations in RpoS present a phenotype that allows the mutant to survive in extended media for an extended time (up to 5 years).

Question 59

Q

What is the phenotype called that allows for a long-term stationary phase?
What do these cells do?
What else is required to allow long-term survival of the culture?

Answer

A

GASP - growth advantage in stationary phase
The GASP cells continue to grow and actually replace each other.
Programmed cell death, initiated by a stress-response, RpoE, is required to allowed long-term survival of the culture.

Question 60

Q

What is Diauxic Growth?

Answer

A

Preferentially growing on one carbon source before using the second carbon source. Most bacteria (r-strategists) need to grow as quickly as possible to try to outcompete other bacteria in the same environment, so they want to use the most energy-efficient carbon source first.

Question 61

Q

Many bacteria grow preferentially on _____.

Answer

A

Glucose when presented with media containing glucose and other carbon sources (such as lactose).

Question 62

Q

Between glucose and lactose, which is more energy-efficient?

Answer

A

Glucose… no extra enzymes to break it down, goes directly into glycolysis. In order to use lactose, the bacteria must produce the enzyme lactase; then lactase breaks lactose into glucose and galactose. This is longer and less efficient.

Question 63

Q

How many lag phases are in Diauxic growth?

Answer

A

There are two lag phases. In the second lag phase, the enzymes needed to utilize the second carbon source are produced.

Question 64

Q

When does catabolite repression occur?

Answer

A

Catabolite repression occurs when one molecule (usually glucose) represses the synthesis of enzymes needed to grow on the second carbon source.

Answer 62

A

Can occur with other C sources, as well as with glucose.

Answer 63

A

“Steady state growth”
Allows continuous growth of cells at controlled rate and density.
Concept: At low nutrient concentration, growth rate is a function of nutrient uptake rate and utilization.

Answer 64

A

D = dilution rate
F = flow rate
V = volume

Answer 65

A

Cell division is the splitting of a mother cell into two daughter cells separated by a septum.

Answer 66

A

When a growing cell reaches a critical mass.

Answer 67

A

During replication, sister chromosomes move toward opposite ends of the cell. Soon after chromosome replication is complete, inward growth of the cell membrane and peptidoglycan for a septum between the two newly replicated chromosomes. Soon after replication, cell separation occurs (in bacteria that grow as single cells).

Answer 68

A

Interval between cell division and initiation of DNA

Answer 69

A

Time between rounds of DNA replication initiation

Answer 70

A

Period of DNA synthesis (genome replication)

Answer 71

A

Period between the end of genome replication and the end of cell division.

Answer 72

A

Total cell cycle = B + C +D

Answer 73

A

DNA replication: DNA replication & Chromosome partitioning
Cell Division: D period

Answer 74

A

Fts proteins. The role of these proteins in bacterial cell division is very complex.

Answer 75

A

FtsZ is a tubulin homolog involved in bacterial cell division.

Answer 76

A

The FtsZ and its associated proteins are called the septal ring.

Answer 77

A

All bacteria and archaea (homolog of tubulin).
The septal ring is not present in a newborn cell or at the end of the cells. If you removed FtsZ, then there would be no septal ring, just a line of cells.
ftsZ mutants form filaments without constrictions.

Answer 78

A

Essential cytoplasmic cell division protein.
Stabilizes the FtsZ protofilaments by cross-linking them.
Serves as a cytoplasmic membrane anchor for the Z ring.
zipA mutant form filaments without constrictions.

Answer 79

A

Probably ATPase - interacts with FtsZ to promote continuation of septum formation.
ftsA mutants form indented filaments but don’t form complete septum.

Answer 80

A

It is imperative that FtsZ ring forms at mid cell.

Answer 81

A

The Min System

Answer 82

A

The Min System regulates central location of FtsZ. The Min System ensures that the mother cell divides into two identically-sized daughter cells.
Nucleoid occlusion and the Min System work together to ensure the Z-ring forms at mid cell.

Answer 83

A

Minicell genetic locus in G- bacteria has three genes: minC, minD, and minE, whose protein products are involved in cell division.

Answer 84

A

MinD forms a cytoplasmic membrane-associated cup at one cell pole that extends toward midcell. It is drawn to the curvature of the cell and binds at one of the two poles.

Answer 85

A

Division inhibitor, inhibits FtsZ from assembly into a Z ring, binds to MinD (MinC cannot directly bind to membrane, must bind to MinD)… MinD has ATPase activity that is required for MinC function.

Answer 86

A

Responsible for topological specificity (ensuring the cell divides at midcell), displaces MinCD complex from one pole & forms a ring that initiates displacement of the MinD cup, MinE will chase MinCD complex from one pole to the other.
MinCD oscillates back and forth to each pole, preventing FtsZ ring from forming.
The only place that FtsZ formation is not being inhibited is at the center of the cell, ensuring you have two equally sized daughter cells.

Answer 87

A

MinE localizes to a ring-like structure in the middle of the cell. The MinCD complex accumulates alternately at the membrane periphery on either side of the MinE ring.
-The MinE ring displaces the MinCD complex at the pole… This oscillation of MinD at each pole occurs very rapidly (seconds) ensures that no FtsZ ring is assembled at either the 1/4 or 3/4 sites of the cell halves.
-The presence of MinE at midpoint prevents MinD inhibitory activity at this site, and allows FtsZ ring assembly in the center.
-The MinE ring disassembles before completion of constriction.

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Lecture 4 - Exam 1 Flashcards

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