We stained inoculated biofilms and performed the Crystal Violet assay. Left in 37 C for 36 hours. We did 4 trials 100uL, 4 trials 200uL, and 4 trials 300uL. Biofilm formation was successful, with varying band thickness. We also replicated this with two 5mL LB petri dish inoculated with 20uL E.coli. We added 5mL of crystal violet each to the petri dishes to cover the whole plate.

We also performed an oxalic acid gradient with 0%, 0.05%, 0.1%, 0.2%, 0.3%, 0.4%, 0.5%, and 2.0% oxalic acid to give a final volume of 6mL. We added 20uL of E.coli to each 6mL tube. Left in 37 C.

We did a 1/100 dilution of E.coli into LB media, and left it in 37 C for (hopefully) 24 hours. We did 4 trials 100uL, 4 trials 200uL, and 4 trials 300uL.

Biofilm produced on 24h 96 well plate.

Testing to see if biofilm will produce on 12h 96 well plate (1 in 100 culture dilution).

And also doing 24h 96 well biofilm formation testing to see what detergents and chemical impacts have on the decrease in biofilm production.

*Biofilms placed at 8:00pm

Oxalic acid test run for 12 hours (0, 0.01, 0.05, 0.1, 0.15, 0.2, 0.4, 0.4, 0.5, 2.0%)

*Oxalic acid placed at 7:30pm

Tested the production of parafilm sacs for in vitro Varroa feeding. (using kimwipes and 2mL tubes as containment methods) .

Performed oxalic acid testing of E.coli growth in LB media at (0, 0.01, 0.05, 0.1, 0.15, 0.2, 0.4, 0.4, 0.5, 2.0%) concentrations. Placed at 6:50pm.

Produced more biofilms.

Had mites and created pouches including Water, LB, Supernatent, E.coli, E.coli RFP. Placed at room temperature and in chris’s drawer.

Took 48 and 24 hour biofilms and performed a bleach treatment on them (0.252%) for 30 minutes. .

Took oxalic acid readings after 23 hours of incubation

Readings are unrealiable as the cultures were left in the shaking incubator for over 23 hours. Still show the same general trend as past gradients.

Make oxalic acid samples again.

Make 24h biofilms.

Objective:

Determine if we have successfully cultured mites in vitro using either paraffin pouches or bee pupae.

Table 2. Experimental design showing each of the treatments applied to the mites.

After 24 hours, all mites were found to be dead. Pupae showed some signs of black bacteria growth or browning on body. Will need to repeat or find another method of culturing mites in vitro.

Biofilm test performed on

Fantastic = Biofilm remained

Windex = Biofilm remained

Bleach = didn’t remain

Made overnight cultures for oxalic acid testing

13 hours left in shaker

Biofilm produced on 24h 96 well plate.

Testing to see if biofilm will produce on 12h 96 well plate (1 in 100 culture dilution).

And also doing 24h 96 well biofilm formation testing to see what detergents and chemical impacts have on the decrease in biofilm production.

*Biofilms placed at 8:00pm

Oxalic acid test run for 12 hours (0, 0.01, 0.05, 0.1, 0.15, 0.2, 0.4, 0.4, 0.5, 2.0%)

*Oxalic acid placed at 7:30pm

Tested the production of parafilm sacs for in vitro Varroa feeding. (using kimwipes and 2mL tubes as containment methods) .