Team:BYU Provo/Notebook/Cholera - Enzyme/May-June/Period1/Dailylog
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+ | : <u> '''Cholera Enzyme''' </u> </font> | ||
: [[Team:BYU Provo/Notebook/Cholera - Enzymes/March-April|March-April]] | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/March-April|March-April]] | ||
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: [[Team:BYU Provo/Notebook/Cholera - Enzymes/September-October|September-October]] | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/September-October|September-October]] | ||
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+ | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/Protocols|Protocols]] | ||
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<font size="4">'''5/3/13'''</font> | <font size="4">'''5/3/13'''</font> | ||
- | We started new cultures of cholera to grow over the weekend. Cultures were prepared in 4mL of our high | + | We started new cultures of cholera to grow over the weekend. Cultures were prepared in 4mL of our high SSW LB. We also streaked our cholera onto a new plate. Both the plate and the overnight cultures were placed in the 30°C incubator to grow over the weekend. |
We heard back from the Lyons, France iGem team about getting part BBa_K802001 from them, however they are on vacation until Monday. They will send us the part as soon as they get back. We emailed them our FedEx shipping number and address. We also checked on the primers that last year's iGem team prepared for the DspB, but they were using a different plasmid vector so we will have to redesign new primers for the part that we are getting so that we can use it in the pet-15B plasmid in order to allow us to easily purify the proteins once we get the gene cloned into E. coli and are producing the enzyme. We will work on designing the new primers this weekend so that we can order them on Monday. | We heard back from the Lyons, France iGem team about getting part BBa_K802001 from them, however they are on vacation until Monday. They will send us the part as soon as they get back. We emailed them our FedEx shipping number and address. We also checked on the primers that last year's iGem team prepared for the DspB, but they were using a different plasmid vector so we will have to redesign new primers for the part that we are getting so that we can use it in the pet-15B plasmid in order to allow us to easily purify the proteins once we get the gene cloned into E. coli and are producing the enzyme. We will work on designing the new primers this weekend so that we can order them on Monday. | ||
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<font size="4">'''5/9/13'''</font> | <font size="4">'''5/9/13'''</font> | ||
- | Today the primers designed for dspB, AmyA, and Savinase were received in the mail. Cholera overnights #1 were seeded and left in the 30 degree incubator. Overnights were made by adding: 4 mL | + | Today the primers designed for dspB, AmyA, and Savinase were received in the mail. Cholera overnights #1 were seeded and left in the 30 degree incubator. Overnights were made by adding: 4 mL SSW LB + 0.5 mL previous cholera overnight. |
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The following is our modified biofilm assay protocol: | The following is our modified biofilm assay protocol: | ||
- | <font size="4">'''Biofilm Assay Protocol'''</font>< | + | |
+ | <div style="text-align:center;"> <font size="4">'''Biofilm Assay Protocol'''</font></div> | ||
'''Biofilm Prep'''<br> | '''Biofilm Prep'''<br> | ||
- | #Overnight culture of V. cholerae grown in | + | #Overnight culture of V. cholerae grown in SSW LB at 30 °C for 72 hrs. |
- | #20 ml of culture added to 180 ml of | + | #20 ml of culture added to 180 ml of SSW LB for dilution |
- | #Fill each well of a 96-well plate with 200 ul of | + | #Fill each well of a 96-well plate with 200 ul of SSW LB |
#To inoculate wells, immerse replicator pins in the diluted bacterial suspension for 30 seconds, then lower replicator pins into wells and agitate for 15 seconds. | #To inoculate wells, immerse replicator pins in the diluted bacterial suspension for 30 seconds, then lower replicator pins into wells and agitate for 15 seconds. | ||
#Plates are covered and incubated with shaking at 30 °C for 24 hrs. | #Plates are covered and incubated with shaking at 30 °C for 24 hrs. | ||
- | #Every 10-12 hrs during the incubation period, spent nutrients are pipetted from wells and replaced with fresh | + | #Every 10-12 hrs during the incubation period, spent nutrients are pipetted from wells and replaced with fresh SSW LB |
'''Enzyme Treatment'''<br> | '''Enzyme Treatment'''<br> | ||
#At 24 hrs, planktonic suspensions and nutrient solutions are aspirated and wells are rinsed by carefully removing and adding liquid from the side of the well using a micropipette. Wells are washed four times. | #At 24 hrs, planktonic suspensions and nutrient solutions are aspirated and wells are rinsed by carefully removing and adding liquid from the side of the well using a micropipette. Wells are washed four times. | ||
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##CV absorbance is read at 540 nm | ##CV absorbance is read at 540 nm | ||
#Each raw absorbance value is then corrected by subtracting the mean of absorbance readings for the blank wells prior to statistical analysis | #Each raw absorbance value is then corrected by subtracting the mean of absorbance readings for the blank wells prior to statistical analysis | ||
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Latest revision as of 23:41, 27 September 2013
Cholera - Enzymes Notebook: May 1 - May 14 Daily Log
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5/1/13 We met today and went over some safety information on working with our BSL2 cholera. We then broke up into our smaller teams to make goals and deadlines for our lab work for the semester. The following is the outline of our goals and deadlines: Goals for Spring Semester:
We have also had difficulties finding a source to obtain our Subtilisin savinase gene, so we may need to order the Subtilisin savinase gene as well. We emailed Dr. Grose the sequence that we need, as well as possible costs from several companies. iGem Teams Contacted: Team Lyon-INSA iGem Contact: lyon.biosciences.igem@gmail.com Part: BBa_K802001 - constitutive promoter (Pveg) + dispersin B gene (dspB)
1 aqsvpwgisr vqapaahnrg ltgsgvkvav ldtgisthpd lnirggasfv pgepstqdgn 61 ghgthvagti aalnnsigvl gvapsaelya vkvlgasgsg svssiaqgle wagnngmhva 121 nlslgspsps atleqavnsa tsrgvlvvaa sgnsgagsis yparyanama vgatdqnnnr 181 asfsqygagl divapgvnvq stypgstyas lngtsmatph vagaaalvkq knpswsnvqi 241 rnhlkntats lgstnlygsg lvnaeaatr Pasted from <http://www.ncbi.nlm.nih.gov/protein/P29600.1>
1 aattgttgcg taaaaggcaa ttccatatat ccgcaaaaaa caagtaccaa gcagaccgga 61 ttaatgctgg acatcgcccg acatttttat tcacccgagg tgattaaatc ctttattgat 121 accatcagcc tttccggcgg taattttctg cacctgcatt tttccgacca tgaaaactat 181 gcgatagaaa gccatttact taatcaacgt gcggaaaatg ccgtgcaggg caaagacggt 241 atttatatta atccttatac cggaaagcca ttcttgagtt atcggcaact tgacgatatc 301 aaagcctatg ctaaggcaaa aggcattgag ttgattcccg aacttgacag cccgaatcac 361 atgacggcga tctttaaact ggtgcaaaaa gacagagggg tcaagtacct tcaaggatta 421 aaatcacgcc aggtagatga tgaaattgat attactaatg ctgacagtat tacttttatg 481 caatctttaa tgagtgaggt tattgatatt tttggcgaca cgagtcagca ttttcatatt 541 ggtggcgatg aatttggtta ttctgtggaa agtaatcatg agtttattac gtatgccaat 601 aaactatcct actttttaga gaaaaaaggg ttgaaaaccc gaatgtggaa tgacggatta 661 attaaaaata cttttgagca aatcaacccg aatattgaaa ttacttattg gagctatgat 721 ggcgatacgc aggacaaaaa tgaagctgcc gagcgccgtg atatgcgggt cagtttgccg 781 gagttgctgg cgaaaggctt tactgtcctg aactataatt cctattatct ttacattgtt 841 ccgaaagctt caccaacctt ctcgcaagat gccgcctttg ccgccaaaga tgttataaaa 901 aattgggatc ttggtgtttg ggatggacga aacaccaaaa accgcgtaca aaatactcat 961 gaaatagccg gcgcagcatt atcgatctgg ggagaagatg caaaagcgct gaaagacgaa 1021 acaattcaga aaaacacgaa aagtttattg gaagcggtga ttcataagac gaatggggat 1081 gagtga Pasted from <http://www.ncbi.nlm.nih.gov/nuccore/ay228551>
5/3/13 We started new cultures of cholera to grow over the weekend. Cultures were prepared in 4mL of our high SSW LB. We also streaked our cholera onto a new plate. Both the plate and the overnight cultures were placed in the 30°C incubator to grow over the weekend. We heard back from the Lyons, France iGem team about getting part BBa_K802001 from them, however they are on vacation until Monday. They will send us the part as soon as they get back. We emailed them our FedEx shipping number and address. We also checked on the primers that last year's iGem team prepared for the DspB, but they were using a different plasmid vector so we will have to redesign new primers for the part that we are getting so that we can use it in the pet-15B plasmid in order to allow us to easily purify the proteins once we get the gene cloned into E. coli and are producing the enzyme. We will work on designing the new primers this weekend so that we can order them on Monday. We are also going to research assay methods for our specific enzymes to be able to test the ability of our enzymes to degrade biofilms. On Monday we will go over the different methods we researched and plan which assays we are going to use for our specific enzymes. We gave the sequence of the Subtilisin savinase gene to Dr. Grose for her to order today. Their turn around time is seven days, then a few extra to mail it to us. We will adjust our goal dates according to when we receive the sequence back.
5/6/13 We talked to Dr. Robison today and were able to get a sample of Bacillus subtilis from his lab. The savinase produced by this bacteria strain is a homolog to the savinase that we were originally looking for. We plated the sample that we got from him and put it in the incubator at 30C to grow the culture. Once the bacteria is grown we can amplify the gene that we want and clone it into the pET15b plasmid to allow us to purify the gene after it is produced, as the pET15b plasmid attaches a His-tag to the protein that causes it to be excreted from the cell and easily isolated and purified.
DspB forward (BI242):
DspB reverse (BI243):
AmyA forward (BI259):
AmyA reverse (BI260):
Subtilisin savinase forward (BI255):
Subtilisin savinase reverse (BI256):
AmyA Degradation:
Alternative seawater medium:
Quantification of Biofilm Biomass:
Papers to consider for enzyme assay/biofilm breakdown:
5/8/13 We are waiting for our primers to get in, but we set up five polyacrylamide gels in preparation for protein assays that we will do in the near future. We also discussed the different papers that we have each researched to find a suitable assay for biofilm degradation analysis. Most of the papers that we found referred back to a 2003 paper for the general protocol followed:
We decided to base our assay off of the protocol presented in this paper, then adjust for our specific needs with cholera. We’ll all go over this paper again in preparation for Friday so we can order the reagents that we will need for this.
5/9/13 Today the primers designed for dspB, AmyA, and Savinase were received in the mail. Cholera overnights #1 were seeded and left in the 30 degree incubator. Overnights were made by adding: 4 mL SSW LB + 0.5 mL previous cholera overnight.
5/10/13 We started a new V. cholerae culture and seeded it from the cultures started on 5/3/2013. The biofilm growth continues to be really good when using our SLB media. We also got our primers back so we will start our pcr and cloning for AmyA and Savinase on Monday. We also compiled the following list of necessary reagents for our enzyme assay. We sent the list to Dr. Grose to see what is available here and what needs to be ordered. We will alter the protocol on Monday to fit our specific needs. Enzyme Assay:
Reagents:
5/13/13 We rechecked our biofilm growth. Allowing the biofilm to grow for 72 hrs in the SLB media gives the highest yield of biofilm in our overnights.
AmyA plasmid for cloning: pIG 86 Followed protocol for phusion PCR of AMyA and Savinase -Sample 2x with each The following is our modified biofilm assay protocol:
Biofilm Assay Protocol
Biofilm Prep
Enzyme Treatment
Absorbance Readings
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