Difference between revisions of "Part:BBa K1298000:Experience"

(iGEM CoBRA 2014)
(Inserted figure 1 & 2)
Line 14: Line 14:
 
<p>Fifth attempt: Dry spun the tubes four times instead of two. This worked and our digested DNA no longer floated out of the wells while pipetting the DNA inside of the wells.</p>
 
<p>Fifth attempt: Dry spun the tubes four times instead of two. This worked and our digested DNA no longer floated out of the wells while pipetting the DNA inside of the wells.</p>
 
*<b>Restriction Digest & Gel Electrophoresis</b>
 
*<b>Restriction Digest & Gel Electrophoresis</b>
 
+
[[File:DigestResultsFromJune14th(Gel).png]]
 
<i>Figure 1: Gel Results of Digestion with Restriction Enzymes on J04450 Plasmids Containing Three Different Chitinase Protein Codes using a 1 Kb Invitrogen Ladder (June 14th 2014)</i>
 
<i>Figure 1: Gel Results of Digestion with Restriction Enzymes on J04450 Plasmids Containing Three Different Chitinase Protein Codes using a 1 Kb Invitrogen Ladder (June 14th 2014)</i>
 
<p>#1: Track It 1 Kb Invitrogen DNA Ladder (the ladder can be found here: http://www.bio.davidson.edu/molecular/Protocols/gels2002/1kbladder.pdf)</p>
 
<p>#1: Track It 1 Kb Invitrogen DNA Ladder (the ladder can be found here: http://www.bio.davidson.edu/molecular/Protocols/gels2002/1kbladder.pdf)</p>
Line 21: Line 21:
 
<p>#4 - #7: These lanes contain digest results for other chitinases (See BBa_K1298001 and/or BBa_K1298002 for more details)</p>
 
<p>#4 - #7: These lanes contain digest results for other chitinases (See BBa_K1298001 and/or BBa_K1298002 for more details)</p>
 
*<b>Ligation</b>
 
*<b>Ligation</b>
 
+
[[File:PcChia1-1.jpg]]
 
<i>Figure 2: Initial Positive Results of Ligation</i>
 
<i>Figure 2: Initial Positive Results of Ligation</i>
 
<p>The right-handed plate with red colonies: Red colonies do not have the desired chitinase sequence.</p>
 
<p>The right-handed plate with red colonies: Red colonies do not have the desired chitinase sequence.</p>

Revision as of 20:25, 24 June 2014

iGEM CoBRA 2014

  • DNA Optimization

The DNA was optimized with Bio Basic Inc.

The original sequence contained illegal cut sites (PstI; ctgca/g)

atgaaatcga tgaagttctc cgcgatggcg atcgccttgc ttacaatggc gacgatgaat ttgtattttg tatctgctga gcaatgcgga cagcaagcag gcggagctct ttgtcccggt ggcttgtgct gcagcaaatg gggatggtgt ggcaacacgg acgcccattg cgggcaggat tgccagagcc aatgcggagg atcgactccc acgcctcctt cacccactcc cggtggacag ggagttgcat ctatcatcac tgaaagcatt ttcaatgagt tattgaagca cagaaacgac gccggttgca aggccagcgg attctacacc tactctgcct tcattgcagc tgccaatgct tttccttcct tcggcaccac cggcgatgtc gctactcgga aaagagagct cgctgctttc tttggccaaa cctcccacga aaccacagga ggatgggcga cagccccaga cggcgcgtac gcgtggggtt attgtttcaa agaggagcaa ggcaatcctc ccgccgagta ctgccaggca acctcccagt ggccctgtgc atctggaaag agatactacg gacgagggcc cgttcaattg tcatggaatt acaactatgg accggccggg aaggcaatcg gattcgatgg cataaacaac cccgacattg ttgctagcga tgccaccgtc tctttcaaga ccgcaatctg gttctggatg accgcccaat ctccgaaacc ttcttgccac gatgtcatga ccgggaaatg gactccgtcc ggcagcgaca gcgccgctgg gagagctgcg ggatatggag cagttaccaa catcatcaac ggcgggctgg agtgcgggaa aggcagtgac tcgaggcagc aggatcgcat cggcttctac aaaagataca gtgacattct tggggtgagc tatggatcaa acctggattg caacaaccag aggcctttcg gcgctgcagt tcaatctgaa gctcgtctta tcaaaaccgt ggtttga

1. TTGTAG

2. CGGCGG

  • Growing

There are no notes to make on the growing techniques or results.

  • Miniprep

First to Third attempt: DNA was not staying inside of the wells, but we did not understand why.

Fourth attempt: Determined that our digested DNA was ‘floating’ out of the wells (and not sinking to the bottom) because we were not dry spinning it enough in this step. The ethanol was still with the DNA after dry spinning, even though it should have been all gone. We concluded that the two dry spins that we were doing was not enough to get rid of the ethanol.

Fifth attempt: Dry spun the tubes four times instead of two. This worked and our digested DNA no longer floated out of the wells while pipetting the DNA inside of the wells.

  • Restriction Digest & Gel Electrophoresis

DigestResultsFromJune14th(Gel).png Figure 1: Gel Results of Digestion with Restriction Enzymes on J04450 Plasmids Containing Three Different Chitinase Protein Codes using a 1 Kb Invitrogen Ladder (June 14th 2014)

#1: Track It 1 Kb Invitrogen DNA Ladder (the ladder can be found here: http://www.bio.davidson.edu/molecular/Protocols/gels2002/1kbladder.pdf)

#2: This is the PcChia 1-1 protein code (BBa_K1298000) inside a pSB1C3 backbone. It was cut with the enzymes EcoRI and PstI, causing the coding region to be removed from the backbone. This leaves two parts, the chitinase code (1017 bp) and the backbone (2070 bp), and there would only be two lines showing up on the gel.

#3: This is the PcChia 1-1 protein code (BBa_K1298000) inside the pSB1C3 backbone. It was cut with only one enzyme (EcoRI), causing the plasmid to be linearized. There is only one part, meaning only one line would show up on the gel.

#4 - #7: These lanes contain digest results for other chitinases (See BBa_K1298001 and/or BBa_K1298002 for more details)

  • Ligation

File:PcChia1-1.jpg Figure 2: Initial Positive Results of Ligation

The right-handed plate with red colonies: Red colonies do not have the desired chitinase sequence.

  • Transformation

This was performed using DH5alpha competent cells, not NEB Top 10-beta cells.

Applications of BBa_K1298000

User Reviews

UNIQ5337963e70d0f512-partinfo-00000000-QINU UNIQ5337963e70d0f512-partinfo-00000001-QINU