ASEPTIC TECHNIQUE Removing inoculum from a broth culture

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Presentation transcript:

ASEPTIC TECHNIQUE Removing inoculum from a broth culture (organisms growing in a liquid medium)

Hold the culture tube in one hand and in your other hand hold the sterilized inoculating loop

Remove the cap of the pure culture tube with the little finger of your loop hand

Keeping the culture tube at an angle, insert the inoculating loop and remove a loopful of inoculum Remove a loopfull of bacteria from your pure culture

Again flame the lip of the culture tube and Replace the cap

flame the lip of the culture tube

Transferring the inoculum into a broth tube Pick up the sterile broth tube and remove the cap with the little finger

flame the lip of the broth tube

Place the loopful of inoculum into the broth and withdraw the loop

Again flame the lip of the tube Replace the cap

Removing inoculum from a plate organisms growing on an agar surface in a petri plate Sterilize the inoculating loop in the flame Lift the lid of the culture plate and stab the loop into the agar away from any growth to cool the loop

Scrape off a small amount of the organisms and close the lid

Inoculating an Agar Slant 1.Label the sterile nutrient agar slant with the source of the culture and your initials. 2. Sterilize the loop. 3. Using appropriate aseptic technique, remove a loopful of broth from the culture tube. 4. Insert the loop into the sterile agar slant tube and starting at the base of the slant, draw the loop up the slant. Do not penetrate the agar. Sterilize the loop. 5. Incubate the slant at 37o C for 24-48 hours. 6. Observe the slant for growth.

Inoculated Agar Slant, after incubation

microorganisms exist in nature as mixed populations(A mixed culture contains two or more bacterial species )However, to study microorganisms in the lab we must have them in the form of a pure culture

assumed to be a pure culture Streak plates allow for the growth of isolated colonies on the surface of the agar. An isolated colony is a colony that is not touching any other colonies and is assumed to be a pure culture .

Using a flame sterilized inoculation loop, spread (streak) the culture over a small area near the edge of the plate (1) using a continuous motion. Flame sterilize the loop and allow it to cool. Turn the plate and spread the bacteria from the end of area (1)across area(2). (You can see the streak marks of the loop in area(1.) Turn the plate in the same direction and spread the bacteria from the end of area (2)across area(3) Turn the plate in the same direction and spread the bacteria from the edge of area (3)across the rest of the plate (area4). Flame sterilize the loop before setting it down.

Streak pattern 1 2 3 4 Bacterial growth pattern Nice isolation!

Place the plate in a 37o C incubator for 24-48 hours.

Quaetrant streak

Contamination of a streak plate results from leaving the plate open too long or not shielding properly with the lid. Correct procedure

Which streak plate culture started as a pure culture. How can you tell? Answer: the one on the right, because all colonies look alike.