How did they measure total cells? (genetics of bacteria)

In summary, the scientists did an experiment to measure how many cells were revertant to the auxotrophic mutation. They used 10^7 survivors and then measured the number of revertants. To measure the total cell count, they used a survival plate with 10^14 survivors. To measure the number of revertants, they used replica plating.
  • #1
outxbreak
30
0
1. About how many cells were plated to count His+ revertant colonies?
How was total cell number determined?




vrf3gk.jpg




I know that the mutation freq was out of 10^7 survivors. So they had to measure the total cell number and come up with 10^7 survivors? But I'm not sure how they got this exact number of 10^7 survivors?

Then to measure His+ revertants I would think they need to plate the same concentration of cells as they did to measure the total cell count?
 
Physics news on Phys.org
  • #2
Answer the second part of the question first, and that should also lead to the answer to the first.

Imagine yourself doing the experiment - what do you actually do in order to get results?
 
Last edited:
  • #3
Hmm well replica plate from the survival plate (his+ min + glu) onto another plate (-his +min +glu)

But I'm really confused as to how every time point had a survival plate with 10^7 survivors? I guess they started with something like 1*1014 cells and mutagenized them with UV... so is the y-axis saying if the survival plate has 10^14 survivors and the mutant plate has 5 mutants then to find the number of actual mutants that you plot set up:

5 mutants/ 10^14 survivors= x mutants/10^7 survivors
x=5*10^-7 mutants per 10^7 survivors..?
 
  • #4
outxbreak said:
Hmm well replica plate from the survival plate (his+ min + glu) onto another plate (-his +min +glu)

But I'm really confused as to how every time point had a survival plate with 10^7 survivors? I guess they started with something like 1*1014 cells and mutagenized them with UV... so is the y-axis saying if the survival plate has 10^14 survivors and the mutant plate has 5 mutants then to find the number of actual mutants that you plot set up:

5 mutants/ 10^14 survivors= x mutants/10^7 survivors
x=5*10^-7 mutants per 10^7 survivors..?

Your questions come with very little context; fortunately these are very common types of experiment for mutagenesis etc. so we can reasonably guess.

You ask about time points. There are no time points in what you have told us. There is a sketch without experimental points of a graph of slightly processed or calculated numbers showing the frequency in the population of revertants from auxotrophy (i.e. his+) as function of uv dose. This is how such data would normally be presented except there would be experimental points.

Survivors and revertants are measured by the number of colonies you get on a plate, which you can count. You don't, and you don't need to, measure every cell in this way - it would take a long time to count 1014 colonies. You typically aim to have of the order of 100 colonies per plate.

So you have to arrange the experiment to have reasonably countable numbers of colonies for the various conditions. You have the advantage of knowing some expected numbers. (When you don't know beforehand what the numbers are, how are you going to do that?)

Are doing this stuff with no laboratory practice? It sounds like either that or you are not connecting these things up with the lab work.

I think replica platings are not needed and do you no good in this case when you are looking for small frequencies. You do everything by dilutions!
 
Last edited:
  • #5
She gave us no other context. :/

In order to measure total survival don't you need to have a survival plate (min+his) and then replica plate these survivors onto the mutant plate (min-his). This ensures that the mutants came from those survivors.

I'm still not sure the total cells to start with.
I would guess 1*1014 cells in a tube.
Mutagenize the cells in this tube with UV dose.
Then plate onto survival plate after a 100,000 fold dilution. If you get 100 cells it means you had 1*107 survivors/109 cells.. I don't know any other way to get 10^7 survivors.
 
  • #6
outxbreak said:
She gave us no other context. :/

In order to measure total survival don't you need to have a survival plate (min+his) and then replica plate these survivors onto the mutant plate (min-his). This ensures that the mutants came from those survivors.
where else can they come from but survivors?
To know the number of survivors, yes you have to plate on min + his.
According to the sketch about 10-5 of his+ revertants not requiring histidine to form colonies are being easily measured.
I think it is obvious that whatever the volumes etc., to see a convenient number of these, you need to dilute them 10-5 less than you do to measure total survivors.
If you measured by replica plating you would have to look at 105 p!ates to see one colony - there is no point in it




outxbreak said:
I'm still not sure the total cells to start with.
I would guess 1*1014 cells in a tube.
Mutagenize the cells in this tube with UV dose.
Then plate onto survival plate after a 100,000 fold dilution. If you get 100 cells it means you had 1*107 survivors/109 cells.. I don't know any other way to get 10^7 survivors.
right
 

Related to How did they measure total cells? (genetics of bacteria)

1. How do scientists measure total cells in bacteria?

Scientists use a process called cell counting to measure the total number of cells in bacteria. This involves using a microscope to view a sample of bacteria and counting the number of cells present.

2. What equipment is needed to measure total cells in bacteria?

To measure total cells in bacteria, scientists typically use a microscope, a counting chamber, and a hemocytometer - a special type of slide used for counting cells. These tools allow for accurate and precise cell counting.

3. Is there a standard method for measuring total cells in bacteria?

Yes, there is a standard method for measuring total cells in bacteria. This method involves diluting a sample of bacteria, placing it on a counting chamber, and then counting the cells present using a microscope. This process is repeated multiple times and the average number of cells is calculated to determine the total cell count.

4. Are there any limitations to measuring total cells in bacteria?

Yes, there are some limitations to measuring total cells in bacteria. One limitation is that the process of counting cells can be time-consuming and requires a skilled technician. Additionally, some bacterial species may be difficult to count accurately due to their small size or clumping together.

5. Why is it important to measure total cells in bacteria?

Measuring total cells in bacteria is important for several reasons. It allows scientists to monitor the growth of bacterial populations, track changes in cell numbers over time, and determine the efficacy of treatments or interventions. It also provides valuable information for understanding the genetics and behavior of bacteria.

Similar threads

How many living cells on Earth?
    • Biology and Medical
Replies
1
Views
869
How to Calculate the Density of Aluminum in a Face-Centered Cubic Unit Cell
    • Biology and Chemistry Homework Help
Replies
2
Views
11K
I The answer is 15! What is the problem?
    • General Math
Replies
1
Views
1K
Did Neurons Evolve from Secretory Cells?
    • Biology and Medical
Replies
2
Views
3K
How many alleles per gene the human species have today?
    • Biology and Medical
Replies
3
Views
2K
Calculating Cell Potential Using Nernst Equation for Ag+ Voltaic Cell
    • Biology and Chemistry Homework Help
Replies
4
Views
5K
I Measurement problem - will this work?
    • Quantum Physics
Replies
3
Views
370
Calculating the Original Concentration of Bacteria
    • Biology and Chemistry Homework Help
Replies
2
Views
15K
In-Flight Incident: My Experience with a Throttle Malfunction | Pilot's Story
    • Aerospace Engineering
Replies
13
Views
816
New CRISPR-based tool for find-and-replace editing of DNA
    • Biology and Medical
Replies
2
Views
3K

Hot Threads

Recent Insights

Back
Top