Star

BBa_K1218026 Version 1

Component

Source:
http://parts.igem.org/Part:BBa_K1218026
Generated By: https://synbiohub.org/public/igem/igem2sbol/1
Created by: Simon Vecchioni
Date created: 2013-09-16 11:00:00
Date modified: 2015-05-08 01:09:42

32bp10CC Duplex Nanowire



Types
DnaRegion

Roles
DNA

sequence_feature

Sequences BBa_K1218026_sequence (Version 1)

Description

Overview:

The 30bp10CC Duplex Nanowire is a produces a silver-chelating/intercalating hairpin nanowire. Silver is taken up by cytosine-cytosine mismatches in the hairpin. Rather than the canonical hydrogen bonds between a purine and pyrimidine, this system uses Ag+ ions to bridge the gap between the N3 sites on opposing pyrimidines. This brick is designed to function in vitro as an extra-cellular BioBrick.

Specs:
??? DNA duplex 32bp in length
??? 10 mismatches, bundled in the center in a 2-1-2 pattern (CCACC???)
??? Will only anneal in the presence of Ag+

Duplex Sequence:
5??? AAA CAT TTA CC A CC T CC T CC A CC T TAT AGT TT 3???
||| ||| ||| ?????? | ?????? | ?????? | ?????? | ?????? | ||| ||| ||
3??? TTG TTA AAT CC T CC A CC A CC T CC A ATA TCA AA 5???

DNA duplex excision:

The brick is packaged with premade primer sequences for PCR. These primers are: F-CCAAGCACGCCCACCT (Tm 59.5⁰C) and R-TGGTAGGTGGCGGTGC (Tm 58.8⁰C). Once amplified, the mismatch-complimentary sequences can be removed using Pme1 blunt-end restriction sites. The two strands abut one another, the first and last four bases of the sequence constituting half of the 8-bp Pme1 cut site. There are three Pme1 sites, one at the beginning of the region, one between the two strands, and one at the end of the region.

Removal of the anti-sense strand can be done by adding a high concentration of an interfering probe and gel extracting the lighter band.

The duplex can now be annealed.

Annealing DNA:

To ensure optimal silver uptake, AgNO3 is added at a 1:1 molarity with CC mismatches. Thus there should be a 10:1 molar ratio between AgNO3 and the DNA product.

The optimal buffer has been experimentally determined to be 10mM MOPS with 100mM NaNO3. In circumstances requiring other buffers (MS, NMR), 10mM ammonium acetate and 10mM phosphate buffer have been substituted for MOPS. Avoid any chelating buffers such as TAE, as this will inhibit silver uptake by the DNA.
Add silver and buffer to the sample, and heat at 90⁰C for 2 minutes, then let cool slowly to room temperature over the course of an hour. For optimal annealing, let cool at 4⁰C for an additional hour prior to experimentation.

Store at -20⁰C for best results.

In sum, to produce the DNA duplex
??? Amplify target region using pre-designed primers
??? Digest with Pme1
??? Target anti-sense with high concentration probe DNA
??? Gel extract desired fragment
??? Anneal product

Experimental notes:

Annealed product gels best in 4% agarose gel made in 10mM MOPS (no NaNO3), or 10% polyacrylamide gel under the same conditions. If using 10bp ladder, run at 4⁰C.

Intercalated silver can withstand isopropanol and ethanol precipitation.

Notes

The part must produce a DNA duplex from a DNA sequence, which requires restriction digest and cleanup.

Source

This part is entirely synthetic.

Sequence Annotation Location Component / Role(s)
F_primer
Pme1 site
Pme1 site
Pme1 site
R_primer
Star strand 1 (template)
Star strand 2 (mismatch compliment)
1,16
37,44
69,76
101,108
109,124
41,72
73,104
feature/primer_binding primer_binding_site
feature/misc sequence_feature
feature/misc sequence_feature
feature/misc sequence_feature
primer_binding_site feature/primer_binding
sequence_feature feature/dna
sequence_feature feature/dna
igem#experience
None
 
igem#sampleStatus
In stock
igem#status
Available
 
synbiohub#ownedBy
user/james
 
synbiohub#ownedBy
user/myers
 
synbiohub#topLevel
BBa_K1218026/1