Difference between revisions of "Part:BBa K3046017"

Revision as of 16:29, 16 October 2019 (view source) Registry (Talk | contribs)		Revision as of 01:32, 22 October 2019 (view source) JMejlsted (Talk | contribs) Newer edit →
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	__NOTOC__		__NOTOC__
	<partinfo>BBa_K3046017 short</partinfo>		<partinfo>BBa_K3046017 short</partinfo>
		+	<html>
		+	This part is the bacterial promoter <a href="https://parts.igem.org/Part:BBa_R0010" target="_blank">BBa_R0010</a> with MoClo level 0 compatible overhangs.
		+	<br><br>
		+	<h3>
		+	<span>Usage and Biology</span>
		+	</h3>
		+	The bacterial promoter can be cut out using the Type IIs restriction enzyme as shown in the figure below. Following this, a promoter following the level 0 promoter + 5' UTR MoClo standard can be inserted and the assembled construct can be used for characterization of the promoter.
		+	<br>
		+	<figure>
		+	<img style="width: 60%; padding:28px;" src="https://2019.igem.org/wiki/images/9/96/T--DTU-Denmark--PromEx.svg" alt="This figure shows a bacterial promoter in front of the fluorescent protein mCherry being replaced by a synthetic promoter when cut with BsaI, thus allowing for expression in our organism." class="safetyfirstimg">
		+	<figcaption>Figure 1: The figure shows the general strategy for replacing the prokaryotic promoter BBa_K3046017 upstream of mCherry with a synthetic promoter using Golden Gate assembly.</figcaption>
		+	</figure>
−	ld	+	<br>
		+	When the bacterial promoter is present in the device, mCherry is expressed in <i>E. coli</i> and not in the target eukaryote, such as <i>Aspergillus niger</i>. When the promoter is exchanged, mCherry is no longer expressed in <i>E. coli</i>, but fluorescence can be observed in the eukaryote.
		+	We have demonstrated this in Figure 2 where a promoter from the <a href="https://2019.igem.org/Team:DTU-Denmark/Part_Collection" target="_blank">LEAP library</a> has been inserted.<br>
−	<!-- Add more about the biology of this part here	+
−	===Usage and Biology===	+	<figure>
		+	<img style="width: 60%; padding:28px;" src="https://static.igem.org/mediawiki/parts/4/49/T--DTU-Denmark--part9_proof.png" class="safetyfirstimg">
		+	<figcaption>Figure 2: The figure two plates with <i>E. coli</i> colonies, with the ones on the left containing the bacterial promoter and the right one containing a synthetic fungal promoter. Note that few red colonies can be seen on the plate on the right, which serves as a quick screening method for correct insertion of the promoter.</figcaption>
		+	</figure>
		+	</html>
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Revision as of 01:32, 22 October 2019

MoClo promoter stand-in This part is the bacterial promoter BBa_R0010 with MoClo level 0 compatible overhangs.

Usage and Biology

The bacterial promoter can be cut out using the Type IIs restriction enzyme as shown in the figure below. Following this, a promoter following the level 0 promoter + 5' UTR MoClo standard can be inserted and the assembled construct can be used for characterization of the promoter.

When the bacterial promoter is present in the device, mCherry is expressed in E. coli and not in the target eukaryote, such as Aspergillus niger. When the promoter is exchanged, mCherry is no longer expressed in E. coli, but fluorescence can be observed in the eukaryote. We have demonstrated this in Figure 2 where a promoter from the LEAP library has been inserted.

Sequence and Features