IGEM:Harvard/2006/DNA nanostructures: Difference between revisions

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Project Overview

Our goal is to design and implement molecular containers, which can be dynamically opened and closed by an external stimulus.
The containers will be implemented as DNA nanostructures, which afford a significant degree of positional control and chemical versatility.
As an initial proof-of-concept, we plan to use our DNA containers to demonstrate controllable activation ("delivery") of anti-thrombin aptamers.
We expect that molecular containers could have several interesting scientific and clinical applications, such as
- Drug and gene delivery
- Bio-marker scavenging (early detection of biomarkers)
- Directed evolution (compartmentalized selections)
- Using multiplexing for combinatorial chemical synthesis
- Capture and stabilization of multiprotein complexes
- Protein folding (chaperones)
- Cell sorting

Working Team Members

Recent Changes

No changes during the given period match these criteria.

@@ Line 1: / Line 1: @@
-{{IGEM H06 DNA nano navbar}}
+<div class="tabs-blue">
+<ul>
+<li id="current">[[IGEM:Harvard/2006/DNA nanostructures|Project Overview]]</li>
+<li>[[IGEM:Harvard/2006/DNA_nanostructures/Designs|Designs]]</li>
+<li>[[IGEM:Harvard/2006/DNA_nanostructures/Notebook|Notebook]]</li>
+<li>[[IGEM:Harvard/2006/DNA_nanostructures/Protocols|Protocols]]</li>
+<li>[[IGEM:Harvard/2006/DNA_nanostructures/Presentations|Presentations]]</li>
+<li>[[IGEM:Harvard/2006/DNA_nanostructures/Literature|Literature]]</li>
+</ul>
+</div>
+<br style="clear:both">
 ==Project Overview==
-*Our goal is to to design and implement molecular containers, which can be dynamically opened and closed by an external stimulus.
+*Our goal is to design and implement molecular containers, which can be dynamically opened and closed by an external stimulus.
 *The containers will be implemented as DNA nanostructures, which afford a significant degree of positional control and chemical versatility.
 *As an initial proof-of-concept, we plan to use our DNA containers to demonstrate controllable activation ("delivery") of anti-thrombin aptamers.
@@ Line 14: / Line 25: @@
 **Cell sorting
-==Container Specs==
+==Working Team Members==
-[[Image:iGEM_harv06_mattspecs.gif]]
+*[[User:TChan|Tiffany Chan]] ([[User_talk:TChan|talk]], [[Special:Contributions/TChan|edits]])
+*[[User:Kfifer|Katherine Fifer]] ([[User_talk:Kfifer|talk]], [[Special:Contributions/Kfifer|edits]])
-==Container Designs==
+*[[User:Vlau|Valerie Lau]] ([[User_talk:Vlau|talk]], [[Special:Contributions/Vlau|edits]])
-<gallery>
+*[[User:Matthewmeisel|Matthew Meisel]] ([[User_talk:Matthewmeisel|talk]], [[Special:Contributions/Matthewmeisel|edits]])
-Image:Igemharv06_Katie_Val_cylinderI.gif|[[IGEM:Harvard/2006/Container Design 1|Design 1]]<br>hexagonal core, separate 1-ply lids
+*[[User:Lhahn|Lewis Hahn]] ([[User_talk:Lhahn|talk]], [[Special:Contributions/Lhahn|edits]])
-Image:Smallcontainerdesign2.jpg|[[IGEM:Harvard/2006/Container Design 2|Design 2]]<br>hexagonal core, separate 2-ply lids
+*TA: [[User:ShawnDouglas|Shawn Douglas]] ([[User_talk:ShawnDouglas|talk]], [[Special:Contributions/ShawnDouglas|edits]])
-Image:Igemharv06_msmrect.png|[[IGEM:Harvard/2006/Container Design 3|Design 3]]<br>rectangular core, continuous 1-ply lids
-Image:Websmallbarrsingleply.jpg|[[IGEM:Harvard/2006/Container Design 4|Design 4]]<br>hexagonal core, separate 1-ply lids
-</gallery>
-==Latch Designs==
-<gallery>
-Image:iGEM_harv06_mattlatch1.jpg |latch1 <br>[[:Media:iGEM_harv06_mattlatch1.jpg|jpg]] | [[:Media:IGEM_harv06_mattlatch1.ai|ai]]
-Image:iGEM_harv06_mattlatch2.jpg |latch2 <br>[[:Media:iGEM_harv06_mattlatch2.jpg|jpg]] | [[:Media:IGEM_harv06_mattlatch2.ai|ai]]
-</gallery>
-==Coding==
-===Existing code===
-*[[IGEM:Harvard/2006/DNA_nanostructures/Designing_DNA_nanostructures|William's code (Python)]]
-==Thrombin-aptamer experiments==
-====Questions / procedures====
-* what percent gel? 10% to 20% polyacrylamide gels, no SDS (but would make for a good control)
-* what incubation conditions?
-* how much protein and DNA? protein at 1 {{um}}, DNA at 2 {{um}}
-* Coomassie stain
-====Experiments====
-{| {{table}}
-| align="center" style="background:#f0f0f0;"|number
-| align="center" style="background:#f0f0f0;"|thrombin
-| align="center" style="background:#f0f0f0;"|aptamer
-| align="center" style="background:#f0f0f0;"|nanotube
-| align="center" style="background:#f0f0f0;"|DNA-stained prediction
-| align="center" style="background:#f0f0f0;"|protein-stained prediction
-|-
-|0||-||-||-||no bands||no bands
-|-
-|1||-||-||+||slow band (nanotube)||no bands
-|-
-|2||-||+||-||fast band (aptamer)||no bands
-|-
-|3||-||+||+||slow band (aptamer-nanotube), traces of fast band (aptamer)||no bands
-|-
-|4||+||-||-||no bands||fast band (thrombin)
-|-
-|5||+||-||+||slow band (nanotube)||fast band (thrombin)
-|-
-|6||+||+||-||medium band (aptamer-thrombin), fast band (aptamer)||medium band (aptamer-thrombin), traces of fast band (thrombin)
-|-
-|7||+||+||+||very slow band (thrombin-aptamer-nanotube), slow band (aptamer-nantotube), traces of fast band (aptamer)||very slow band (thrombin-aptamer-nanotube), medium band (aptamer-thrombin), traces of fast band (thrombin)
-|-
-|}
-====Buffers====
-* Macaya's and Bock's selection buffer: 20 mM Tris-acetate, pH 7.4, 140 mM NaCl, 5 mM KCl, 1 mM CaCl<sub>2</sub>, 1 mM MgCl<sub>2</sub>
-* Liu's incubation buffer: 40 mM Tris, 20 mM CH<sub>3</sub>COOH, 2mM EDTA, 12.5 mM (CH<sub>3</sub>COO)<sub>2</sub>Mg, pH 8.0
-* Liu's PAGE buffer: 1x TAE/Mg<sup>2+</sup>
-====Protocols====
-Potential protocol for a 2 {{ul}} incubation reaction (revised with Dr. Shih's suggestions)
-* Reconsitute lyophilized [http://www.sigmaaldrich.com/catalog/search/ProductDetail/SIAL/T6634 bovine thrombin] — ''[[User:Matthewmeisel/Notebook/2006-7-11|done]]''
-* In a 0.2 mL PCR tube, mix:
-** 0.5 {{ul}} of 4x (not 5x) [[IGEM:Harvard/2006/Stock_solutions#Bock.27s_selection_buffer|Bock's selection buffer]]
-** 1.0 {{ul}} of 2 {{um}} aptamers (final concentration: 1.0 {{um}} = 2 pmol)
-** 0.5 {{ul}} of 2 {{um}} thrombin (final concentration: 0.5 {{um}} = 1 pmol)
-* OR in a 0.2 mL PCR tube, mix:
-** 0.5 {{ul}} of 4x (not 5x) [[IGEM:Harvard/2006/Stock_solutions#Bock.27s_selection_buffer|Bock's selection buffer]]
-** 0.5 {{ul}} of 2 {{um}} aptamers (final concentration: 0.5 {{um}} = 1 pmol)
-** 1.0 {{ul}} of 2 {{um}} thrombin (final concentration: 1.0 {{um}} = 2 pmol)
-* Alternative mix: Liu uses 10 pmol of DNA (1 {{ul}} of 10 {{um}}) and varies thrombin amount from 2 pmol (1 {{ul}} of 0.2x thrombin working stock) to 100 pmol (1 {{ul}} of 10x thrombin working stock)
-* Incubate at room temperature for 30 min.
-* Load onto a non-denaturing polyacrylamide gel (10% to 20% gradient) at 4{{c}}
-** Liu runs at 25 mA for 48 h.
-[[User:Matthewmeisel|Matthewmeisel]] 11:11, 11 July 2006 (EDT)
-====Bibliography====
-<biblio>
-# tha1 pmid=8107090
-# tha2 pmid=15945116
-# tha3 pmid=8298130
-# tha4 pmid=1741036
-# tha5 pmid=8475124
-</biblio>
-==Presentations==
-===Most recent (Week 3)===
-* [[Media:IGEMHarv06 Week3 presentation VKTM2.ppt|Week 3 Presentation: Design Progress]]
-===Week 2: Original proposal===
-* [[IGEM:Harvard/2006/DNA_nanostructures/Presentation_proposal|Presentation Proposal]]
-==Working Team Members==
+==Recent Changes==
-*[[User:TChan|Tiffany Chan]] ([[User_talk:TChan|talk]])
+{{Special:Recentchanges/b=IGEM:Harvard/2006/DNA_nanostructures/&limit=20}}
-*[[User:Kfifer|Katherine Fifer]] ([[User_talk:Kfifer|talk]])
-*[[User:Vlau|Valerie Lau]] ([[User_talk:Vlau|talk]])
-*[[User:Matthewmeisel|Matthew Meisel]] ([[User_talk:Matthewmeisel|talk]])
-*...and others are welcome!

IGEM:Harvard/2006/DNA nanostructures: Difference between revisions

Latest revision as of 01:15, 29 October 2006

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