3. แล้วทำการ Streak เชื้อที่อยู่ปลา

3. then follow the Streak end loop fuel onto a Petri dish with agar, who has already prepared with care, which includes the following steps.Petri dish, cover, 3.1, there are enough spaces that are easy to access loop, as shown in Figure 1-7 (a), and complies with Loop that bacteria are making streak at no. 1 by area during the streak will not make the food's surface crack.3.2 when the streak at no. 1, and the area, leading the Loop came out sterilization by flames after it makes a loop cooling by tapping on the edge of the area near the agar No. 1.Petri dish rotation 3.3, is in the appropriate position for the number 2 and then streak area make cross streak by beginning to address that area number 1, and then run the Streak at no. 2 area as shown at. 1-7 (b).3.4 when streak area number 2, leading the Loop came out sterilization by flames after it makes a loop cooling by tapping on the edge of the area near the agar No. 2.Petri dish, rotating 3.5 is in the appropriate position for the streak, and then no. 3 area make cross streak by beginning to address that area number 2 and then make a Streak in which the area number 3 images. 1-7 (b), if necessary, can make the streak area No. 4.3.6 mixtur back Petri and curing, curing the infection in a temperature-controlled Cabinet is 37 degrees Celsius. Long time 24-48 hours, and then observed the growth of pathogens.

3. Then Streak infection in the loop on Petri dishes containing agar was prepared. With caution Steps are as follows:
3.1 Open Petri dishes with enough space to insert easily into the loop. As shown in Figure 1-7 (a), insert the Loop with bacteria is the number one area that streak by the streak will not make a difference of
3.2 on a streak area number one, remove the Loop. out disinfected by fire. After making a loop by tapping on the edge of the agar nearby. No. 1 with a
3.3 plates spinning in the right position for the streak area number 2, then cross streak by beginning to address the number one area then the Streak area No. 2 Figure 1. 7 (b)
3.4 to streak the area number 2, remove the Loop was sterilized by fire. After making a loop by tapping on the edge of the agar nearby. No. 2 with a
3.5 plates spinning in the right position for the streak area number 3 and then cross streak by beginning to address the area No. 2, then No. 3 Streak the area shown in Figure 1. 7 (b) if necessary, can streak the area number 4 has
returned 3.6 Petri dishes and then incubated in a controlled incubation at 37 ° c for 24-48 hours, and then observing the growth of bacteria.

3. Then the Streak infections at the end of the loop onto a Petri dish containing medium has been prepared and with care, the steps are as follows.3.1 open Petri dish to have enough space to insert the loop into easily, as shown in the picture 1-7 (a) then insert Loop contains bacteria are analyzed. Streak area number 1 by during the streak must not make the skin of the food is broken.3.2 when streak that area and the number 1 Loop out disinfection by burning fire, then make loop cool down by tapping at the edge of the medium near. With the number 1.3.3 rotating Petri dish in the proper position for streak area and the number 2 cross streak by beginning to be in area and the number 1 The number Streak area 2 as figure 1-7 (b).3.4 when streak that area and the number 2 Loop out disinfection by burning fire, then make loop cool down by tapping at the edge of the medium near. With the number 2.3.5 rotating Petri dish in the proper position for streak area and the number 3 cross streak by beginning to be in area and the number 2 The number Streak area 3 as figure 1-7 (b) if necessary can be streak at number 4 area.3.6 back Petri dish was incubated curing cabinet temperature control 37 DEG C for 24-48 hours and observe the growth of bacteria.