Subject: Experiment Flowchart of Bacterial Activation and Phage Treatment of Biofilm Formation Style: Concise, scientific experimental flowchart, black lines on a white background, clear icons Requirements: Use clear arrows to connect each step. All key nouns must be represented by icons/pictures, and ensure the icons are easy to understand. The process layout is from left to right and from top to bottom, with clear logic. Steps and Icon List: Start [Icon: Stock tube] (containing target bacteria) Use [Icon: Inoculation loop] to pick up bacterial solution from [Icon: Stock tube]. Perform [Icon: Streak plating] on [Icon: 90mm petri dish] (containing solid medium) to activate bacteria. Incubate in an incubator until [Icon: Single colony] grows. Use [Icon: Inoculation loop] to pick a [Icon: Single colony]. Inoculate the picked colony into [Icon: Erlenmeyer flask] containing [Icon: 2216E liquid medium] and shake culture. Measure periodically until [Icon: Spectrophotometer] shows the bacterial solution [Icon: OD600=0.1]. Branch point: Dispense the bacterial solution into two new, sterile [Icon: Erlenmeyer flasks]. Control group: Keep one [Icon: Erlenmeyer flask] as is. Experimental group: Add [Icon: Bacteriophage] to the other [Icon: Erlenmeyer flask]. Use [Icon: Pipette] to transfer the liquid from the two Erlenmeyer flasks to the wells of 4 [Icon: 24-well plates] respectively (the liquid from each Erlenmeyer flask corresponds to 2 well plates). Parallel processing: Place these 4 [Icon: 24-well plates] in [Icon: Different environments] (e.g., different temperatures or shakers) and incubate for [Icon: 24 hours]. After incubation, remove all well plates. Collect the [Icon: Biofilm] formed in each well plate. Place the collected [Icon: Biofilm] samples in [Icon: 1.5ml centrifuge tube]. End (for subsequent analysis). Layout: Please ensure that steps 1-7 are arranged vertically, and after step 8 (dispensing), the control group and the experimental group expand downwards in parallel, and steps 9-13 converge again.
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