Team:MIT/Organizational Daily Notebook

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Home	The Team	The Project	Parts Submitted to the Registry	Modeling	Notebook

BRAINSTORMING

PROTOCOLS

[http://openwetware.org/wiki/MIT_iGEM_T4_and_Quick_Ligation DNA Ligations]
[http://openwetware.org/wiki/MIT_iGEM_Top10_ChemComp_Ecoli_transformation_protocol#Regular_Transformation_protocol_for_Top10_cells Top10 chem competent cell transformation]
[http://web.mit.edu/biopolymers/www/DNA.html DNA sequencing]
[http://openwetware.org/wiki/Endy_pcr PCR]
[http://openwetware.org/wiki/MIT_iGEM_Agarose_Gels Running DNA Gels]
[http://openwetware.org/wiki/MIT_iGEM_Restriction_Digests Restriction Digests]
[http://openwetware.org/wiki/Endy:Preparing_Antibiotic_Stocks Preparing Antibiotic Stocks]

JUN 10

File:System diagram pic.jpg

JUN 16

Summary of individual tasks to research:

S. Mutans metabolism pathway-Asad
L. bulgaricus metabolism pathway-Allin
secretion (full or partial)-John
other secretion systems (introduction of)-Sara
T7 as a promoter (L. bulgaricus)-Prarthna
L. bulgaricus transformation/protocols-Derek
binding assay protocols-Andrew

Linear Sequence/Design

Ex-promoter-RBS-ATG-signal-epitope-p1025-linker (TEV cleavage site)-GFP-His-TAATAA-termination-SP (see top of page)

Base pairs: 35-10-3-90-30-60-45-700-15-6-8
potential eptiopes
- FLAG (Asp-Tyr-Lys-Asp-Asp-Asp-Asp-Lys)
- C-myc (E Q K L I S E E D L)
- HA (Y P Y D U P D Y A: #2)

DNA/Plasmid Editor

http://www.biology.utah.edu/jorgensen/wayned/ape/

Peptide Sequence Manipulations

http://slam.bs.jhmi.edu/gd/

Primer Analyzer Tool (check temperature & GC content)

http://www.idtdna.com/analyzer/Applications/OligoAnalyzer/Default.aspx

primers should be 17-28 bases in length;
base composition should be 50-60% (G+C);
primers should end (3') in a G or C, or CG or GC: this prevents "breathing" of ends and increases efficiency of priming;
Tms between 55-80oC are preferred;
3'-ends of primers should not be complementary (ie. base pair), as otherwise primer dimers will be synthesised preferentially to any other product;
primer self-complementarity (ability to form 2o structures such as hairpins) should be avoided;
runs of three or more Cs or Gs at the 3'-ends of primers may promote mispriming at G or C-rich sequences (because of stability of annealing), and should be avoided.

- http://bioweb.uwlax.edu/GenWeb/Molecular/Seq_Anal/Primer_Design/primer_design.htm

Parts/Construction

Construction
1. GFP
2. Synthetic peptide
3. L. bulgaricus vector
Assay
L. bulgaricus
S. Mutans

To Do/To Buy:

finalize DNA sequence
primer
synthesis
reagents

TEV Protease cut site

Amino Acid Sequence : Glu-Asn-Leu-Tyr-Phe-Gln-Gly (Cuts between Gln-Gly)
Base Pair Sequence: GAAAACCTGTACTTCCAGGGT

JUN 17

Links to sites from individual research topics

T7 as a promoter in L. bulgaricus/Other viable promoter options
- LacS promoter
  - http://www.patentstorm.us/patents/5639644/description.html
  - http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=161534
- http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=123959
- http://jb.asm.org/cgi/content/full/184/4/928
Secretion signal peptide
- [http://www.pubmedcentral.nih.gov/picrender.fcgi?artid=178052&blobtype=pdf cleavage site]

P4 Revised

File:P4-4.jpg

- reverse sequence: CTG CAG CGG CCG CTA CTA GTA AGA GAA TAT AAA AAG CCA GAT TAT TAA TCC GGC TTT TTT ATT ATT TTT ATT AGT GGT GAT GGT GAT GAT GTT TGT ATA GTT CAT CCA TGC
- length = 111 bp
- melting temp = 69.6 C
- GC content % = 36.0

JUN 18

[[../lbulgaricus |Lactobacillus delbrueckii subsp. bulgaricus Information & Protocols]]

[[../toothbindingassay | Tooth binding assay protocol]]

http://www.freewebs.com/naguiar/ (S. mutans Information)

http://pubs.acs.org/cgi-bin/abstract.cgi/jafcau/2002/50/i05/abs/jf010958t.html (S. mutans adsorption to HA Beads)

http://www.blackwell-synergy.com/doi/full/10.1111/j.1399-302X.2007.00412.x (Influence of Starch and Sucrose on S. mutans)

Friday Meeting breakdown

Andrew: primers
Derek: L. bulgaricus procedures
Allin: metabolism
John: binding assay
Sara: secretion
Asad: S. Mutans/Binding Assay
Prarthna: promoters

JUN 20

Powerpoint [linked here]

JUN 24

Ordered MRS broth and agar for L.bulgaricus from Difco

AUG 1

Initial outline for powerpoint:

1. Overview

  Large synthetic biology -> food overview
  Our goal
  Why important
      Teeth
      Globally
  Plan of Attack
  	forming DNA

lactobacillus bulgaricus binding assay

2. Binding Assay

  New method
      (Controls to prove eficacy of method)

3. DNA work

  Gene construct
  	Brief reason for parts in teh construct

signal seq for l.bulgaricus Promoter characterizing bad T7 BioBricks

4. L.bulgaricus

  Transforming

Restriction Mechanism Emphasize how hard it is

5. Final results

6. Our contribution (biobricks, l.bulgaricus, binding assay for cells)

7. Final overview

   This is specific, but applies to a lot strains / peptides

Home	The Team	The Project	Parts Submitted to the Registry	Modeling	Notebook

@@ Line 128: / Line 128: @@
 ==JUN 24==
 *Ordered MRS broth and agar for L.bulgaricus from Difco
+==AUG 1==
+*Initial outline for powerpoint:
+. Overview
+   Large synthetic biology -> food overview
+   Our goal
+   Why important
+       Teeth
+       Globally
+   Plan of Attack
+   	forming DNA
+	lactobacillus bulgaricus
+	binding assay
+. Binding Assay
+   New method
+       (Controls to prove eficacy of method)
+. DNA work
+   Gene construct
+   	Brief reason for parts in teh construct
+	      signal seq for l.bulgaricus
+	Promoter
+		characterizing bad T7
+	BioBricks
+. L.bulgaricus
+   Transforming
+	Restriction Mechanism
+	Emphasize how hard it is
+. Final results
+. Our contribution (biobricks, l.bulgaricus, binding assay for cells)
+. Final overview
+    This is specific, but applies to a lot strains / peptides