Very helpful videos .... please make video on molecular technics ...PCR , RT-PCR, Nano drops , Sequencing, Electrophoresis,ELISA, Chromatography, spectrophotometry
if your trying to determine the bacterial resistance to a particular antibiotic using serial dilution and total viable count what are the acceptable counts and what are not the acceptable counts to say whether or not bacterial resistance is taking place?
@@rbrlifescience Yes!! we hv used Bushnell Hass agar as a selective medium for the isolation of hydrocarbon degrading bacteria. We did ur dilution technique. Thank you 💯🙏👍
Generally soil contains organic materials so it will have large number of bacteria. To get isolated colonies it is better to take 1 gm of soil. It's an assumption. It's not as per SOP
What about other plates in which we got countable growth how can we include those in calculation and we usually take duplicate or triplicate how can we calculate in such case
suppose you have plated 0.1 ml of sample of 10^3, 10^4, 10^5 dilution on three different plates. suppose you got 100 colony on 10^3 dilution, 11 colony on 10^4 dilution, 2 colony on 10^3 dilution, first conver the count cfu/ 0.1 ml to cfu/ml 10^3 (100 colonies) = 100 x 10^3 cfu/ 0.1 ml = 100 x 10^4 cfu/ ml 10^4, (11 colonies) = 11 x 10^4 cfu/ 0.1 ml = 11 x 10^5 cfu/ ml 10^5 (2 colonies) = 2 x 10^5 cfu/ 0.1 ml = 2 x 10^6 cfu/ ml now convert these 3 result to one specific dilution result 10^3 (100 colonies) = 100 x 10^4 cfu/ ml = 100 x 10^4 cfu/ml 10^4, (11 colonies) = 11 x 10^5 cfu/ ml = 110 x 10^4 cfu/ ml 10^5 (2 colonies) = 2 x 10^6 cfu/ ml = 200 x 10^4 cfu/ ml then average it (100+110+200)/3 = 136.66 x 10^4 cfu/ ml 136.66 x 10^4 cfu/ ml present in your original undiluted sample In the case of duplicate or triplicate samples, just average the results of specific dilution.
Is this method according to iso? I lately worked in a lab wich they consider an inoculum of 0.1 ml from dilution 1/10 as a1/100 dilution on Petri dish Is that right? I could not understand it because they only spread the inoculum & not diluting it. Please I want an answer.
@@rbrlifescience Thank you for replying. But your yes belongs to which part of my question? Is spreading 0.1 ml of dilution 1/10 on a solid culture medium becomes 1/100? Would you please briefly explain it? Or give me a link or any reference?
What about if the 2 plates from 2 different dilution ( 10^2 and 10^3 for example) have colonies within the range of 30-300. What dilution should be consider to calculate the CFU/mL in the undiluted sample
@@rbrlifescience Thank for your explanation. But while performing dilutions there is a possibility that the anaerobic bacteria will come in contact with oxygen and the bacteria will die.So in order to protect anaerobic bacteria to get in contact with oxygen while dilutions, what precautions we have to take?
@@sumitm8904 Dear sumit I totally agree with you. Generally any work on anaerobic bacteria should be carried out in anaerobic chamber. This chamber is purged with nitrogen and Carbon dioxide gas so all oxygen is removed from the chamber. Initially everything apparatus such as plate pouring, dilution making is done inside this chamber. and after plating plate is also placed in anaerobic CO2 incubator. It's little bit difficult to work with obligate anaerobic bacteria. There are different types of anaerobic media such as semisolid media which you can inoculate such bacteria.
As per my opinion fungal samples should be blended in specific broth medium before making dilutions. The procedure of serial dilution in similar as described in video.
@@rbrlifescience Sir maine BSc (BZC) se ki hai , mujhe ,Media preparation, Autoclave operation, Watter sampling and testing, MLT testing ati hai kya mai microbiologist ban sakta hu plzz btaye ,ya apna no. Share kar dijiye taki me apse kuchh puchh saku
@@mishraratnesh6426 Dear Ratnesh if you are a life science student then you can do the job of microbiology. If you have good knowledge of microbiology then there is no problem of getting job in the field in the microbiology. I am postgraduate in Zoology but right now i am working in microbiology field. So cheers.
Suppose you added 1 gm soil in 50 ml of Distilled water/ saline Now you are taking 1 ml of this sample and serially diluting it. You took 0.1 sample of each diluted tube and plated it. Suppose after plating 0.1 ml of sample of tube having dilution 10^-3 (ten power minus three ) you got 10 Colonies. Now it's 10 colonies in 0.1 ml of tube with dilution 10^-3 So convert it to ml 10 × 10= 100 × 10^3 cfu per ml So in 1 ml cfu count is = 100× 10^3 Multiply it by 50 = 100×50 × 10^3 = 5000×10^3 Cfu present in 1 gm of original soil sample Please watch my video on how to calculate CFU/ml
a single bacteria will multiply a number of times and then only we are able to see a single colony. A single bacterial colony is made up of thousands of bacteria that arise by multiple cell division of single cell only.
Dear Sneha initiatilly we calculated how much bacteria we got in 0.1 ml of sample. for plating we generally take out 0.1 ml of sample. once you calculate how many cfu in 0.1 ml of sample then we are simply converting it into 1 ml. multiply (0.1 ml X 10 )= 1 ml thats why we need to multiply cfu present in 0.1 ml with 10 and we will get cfu/ml.
सुरक्षेच्या कारणास्तव मी तुम्हाला माझा मोबाईल नंबर देऊ शकत नाही जर तुम्हाला काही सहकार्य हवे असल्यास तुम्ही कमेंट करू शकता आणि मी त्याचा रिप्लाय तुम्हाला देईन
Finally, find the authentic content
Thanks for watching this video...Stay tuned to watch such more videos
Mind blowing
Thank you
thank you sir for this detailed explanation!
Thank you and stay tuned
Realy so nice explanation 😮
Glad you liked it
Sir, we say thank u so much sir.i require like this teaching sir . 😊🙏🙏🙏🙏🙏🙏🙏
Thank you and please suggest such topics on which I should make videos
Informative Video with excellent explanation.
Thank you Deepak..and stay tuned to watch such more informative videos... 👍😃
Thank you very much sir for this great explanation ❤
Most welcome
Sir very very good lacture for concept and understanding ☺️🤗 this method ♥️👌
Thank you dilawar Khan ji...
really helpful 👌 👏
Nice explanation sir thank you sir for wonder full explanation
Thanks harshada
Best video on CFU❤
Thank You. ....and please suggest any topics on which I should make videos
Good explain sir...J. Cappuccino😊
Welcome sir
Finally,well explained
Thankyou so much sir for making my concept very clear...
Most welcome Deep ...Please also suggest some concepts on which I should make videos
Thank you. It was very educative.
One question. Why would we need to find out the number of cells? In what research do we need it?
To see the growth pattern of bacteria in culture we need to count cells.
Perfect 👍
Thanks 👍
Great knowledge
Thank You
So nice
Very good explanation sir
Thank you madam and please suggest any topics on which I should make videos
❤❤❤ ⚘️🌷⚘️...Thank you...🙏🙏😊😊😊👍👍👍
Most welcome
excellent explanation...thanks..
Most welcome and stay tuned for more videos
Very helpful videos .... please make video on molecular technics ...PCR , RT-PCR, Nano drops , Sequencing, Electrophoresis,ELISA, Chromatography, spectrophotometry
Thank you for suggestions...I will definitely make videos on molecular techniques
Tq sir
Welcome
Pls sir do you have any video on complete method for culturing bacteria
Please explain in detail
No words😊😊😊
Good sir from pakistan
Most Welcome
Very helpful vedio thank you
Thank you madhu....let me know other topics on which you want such videos
very nice
Thank you
thank you
most welcome
if your trying to determine the bacterial resistance to a particular antibiotic using serial dilution and total viable count what are the acceptable counts and what are not the acceptable counts to say whether or not bacterial resistance is taking place?
Please go through this wic.oregonstate.edu/microbiology-writing-guide-presenting-data
Thanks
Welcome
Will this dilution technique useful for oil contaminated soil ?
Yes, off course but you have to choose correct medium of agar plates for plating as per type of microorganisms
@@rbrlifescience Yes!! we hv used Bushnell Hass agar as a selective medium for the isolation of hydrocarbon degrading bacteria. We did ur dilution technique. Thank you 💯🙏👍
Most welcome mitali @@mitalibhoir6380
K I got it!
Why 1grm of soil in 50ml water?. Is dis jt an assumption or it's from an SOP?
Generally soil contains organic materials so it will have large number of bacteria. To get isolated colonies it is better to take 1 gm of soil. It's an assumption. It's not as per SOP
Which tubes have present actinomycete, bacteria?
It depends on samples
290× 103 and 32×104 how To calculate them?
First convert 290x 10^3 = 29x10^4
Now take average of both
29x10^4
32x10^4
------------------
Answer is 30.5 x 10^4
What about other plates in which we got countable growth how can we include those in calculation and we usually take duplicate or triplicate how can we calculate in such case
suppose you have plated 0.1 ml of sample of 10^3, 10^4, 10^5 dilution on three different plates. suppose you got 100 colony on 10^3 dilution, 11 colony on 10^4 dilution, 2 colony on 10^3 dilution,
first conver the count cfu/ 0.1 ml to cfu/ml
10^3 (100 colonies) = 100 x 10^3 cfu/ 0.1 ml = 100 x 10^4 cfu/ ml
10^4, (11 colonies) = 11 x 10^4 cfu/ 0.1 ml = 11 x 10^5 cfu/ ml
10^5 (2 colonies) = 2 x 10^5 cfu/ 0.1 ml = 2 x 10^6 cfu/ ml
now convert these 3 result to one specific dilution result
10^3 (100 colonies) = 100 x 10^4 cfu/ ml = 100 x 10^4 cfu/ml
10^4, (11 colonies) = 11 x 10^5 cfu/ ml = 110 x 10^4 cfu/ ml
10^5 (2 colonies) = 2 x 10^6 cfu/ ml = 200 x 10^4 cfu/ ml
then average it (100+110+200)/3 = 136.66 x 10^4 cfu/ ml
136.66 x 10^4 cfu/ ml present in your original undiluted sample
In the case of duplicate or triplicate samples, just average the results of specific dilution.
How can we will perform serial dilution method for tonsils sample after tonsillectomy for bacteria identification?
please refer medical procedure, I am explained only general procedure
Is this method according to iso?
I lately worked in a lab wich they consider an inoculum of 0.1 ml from dilution 1/10 as a1/100 dilution on Petri dish
Is that right? I could not understand it because they only spread the inoculum & not diluting it.
Please I want an answer.
Yes it is but you have to do literature survey
@@rbrlifescience Thank you for replying. But your yes belongs to which part of my question?
Is spreading 0.1 ml of dilution 1/10 on a solid culture medium becomes 1/100?
Would you please briefly explain it? Or give me a link or any reference?
microbenotes.com/serial-dilution/
@@rbrlifescience Thank you so much.
What about if the 2 plates from 2 different dilution ( 10^2 and 10^3 for example) have colonies within the range of 30-300. What dilution should be consider to calculate the CFU/mL in the undiluted sample
Yes thats very correct
Can we use this method for counting the anaerobic bacteria ?
You can make dilutions and then do pour plate method to count the anerobic bacteria. There are anaerobic jars in which you have to incubate plates.
@@rbrlifescience Thank for your explanation. But while performing dilutions there is a possibility that the anaerobic bacteria will come in contact with oxygen and the bacteria will die.So in order to protect anaerobic bacteria to get in contact with oxygen while dilutions, what precautions we have to take?
@@sumitm8904 Dear sumit I totally agree with you. Generally any work on anaerobic bacteria should be carried out in anaerobic chamber. This chamber is purged with nitrogen and Carbon dioxide gas so all oxygen is removed from the chamber. Initially everything apparatus such as plate pouring, dilution making is done inside this chamber. and after plating plate is also placed in anaerobic CO2 incubator. It's little bit difficult to work with obligate anaerobic bacteria. There are different types of anaerobic media such as semisolid media which you can inoculate such bacteria.
Sir how to make different concentrations of the fungus
As per my opinion fungal samples should be blended in specific broth medium before making dilutions. The procedure of serial dilution in similar as described in video.
Sir mai aap se kuchh puchna chahta hu plzzz reply dijiye
yes bro
@@rbrlifescience Sir maine BSc (BZC) se ki hai , mujhe ,Media preparation, Autoclave operation, Watter sampling and testing, MLT testing ati hai kya mai microbiologist ban sakta hu plzz btaye ,ya apna no. Share kar dijiye taki me apse kuchh puchh saku
@@mishraratnesh6426 Dear Ratnesh if you are a life science student then you can do the job of microbiology. If you have good knowledge of microbiology then there is no problem of getting job in the field in the microbiology. I am postgraduate in Zoology but right now i am working in microbiology field. So cheers.
Sir ap contact no denge kya ?
@@mishraratnesh6426 yes you can call me 9673690563 either on Saturday and Sunday
How to know the number of bacteria in original soil sample... We added 1 g in 50 ml... How to know the number of bacteria from that 1 g of soil ...
Suppose you added 1 gm soil in 50 ml of Distilled water/ saline
Now you are taking 1 ml of this sample and serially diluting it.
You took 0.1 sample of each diluted tube and plated it.
Suppose after plating 0.1 ml of sample of tube having dilution 10^-3 (ten power minus three ) you got 10 Colonies.
Now it's 10 colonies in 0.1 ml of tube with dilution 10^-3
So convert it to ml
10 × 10= 100 × 10^3 cfu per ml
So in 1 ml cfu count is = 100× 10^3
Multiply it by 50
= 100×50 × 10^3
= 5000×10^3
Cfu present in 1 gm of original soil sample
Please watch my video on how to calculate CFU/ml
How to do of average figures?
All dilution must be the same
Après on fait la moyenne ?
Sir , is it true that single colony produce by single bacteria
a single bacteria will multiply a number of times and then only we are able to see a single colony. A single bacterial colony is made up of thousands of bacteria that arise by multiple cell division of single cell only.
👋
Welcome
That's how homeopathy works. Or doesn't.
32×103 should be divided by 10 not multiplied by it..I guess
Dear Sneha initiatilly we calculated how much bacteria we got in 0.1 ml of sample.
for plating we generally take out 0.1 ml of sample.
once you calculate how many cfu in 0.1 ml of sample then we are simply converting it into 1 ml.
multiply (0.1 ml X 10 )= 1 ml
thats why we need to multiply cfu present in 0.1 ml with 10 and we will get cfu/ml.
@@rbrlifescience thank you so much for clarifying..
@@sneha-zb1yg most welcome and please suggest any topic or concept on which video is required.
@@rbrlifescience if possible please make vedio on plaque assay, and protein-protein interaction techniques..
Hello sir
Hello, Good Morning
Rahul sir no send kara
सुरक्षेच्या कारणास्तव मी तुम्हाला माझा मोबाईल नंबर देऊ शकत नाही जर तुम्हाला काही सहकार्य हवे असल्यास तुम्ही कमेंट करू शकता आणि मी त्याचा रिप्लाय तुम्हाला देईन
Ok sir
May I know which subject or degree you are studying?