Difference between revisions of "Part:BBa K3046006"

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	<partinfo>BBa_K3046006 short</partinfo>		<partinfo>BBa_K3046006 short</partinfo>
−	[[File:T--Valencia_UPV--GFP_spectrum.png|900px|thumb|none|alt=GFP spectra.|Figure 1. GFP emission and excitation spectra]]	+	This is a synthetic constitutive promoter, created as part of the LEAP (Library of Engineered Aspergillus Promoters) project
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−	<!-- Add more about the biology of this part here
	===Usage and Biology===		===Usage and Biology===
		+	This is a weak constitutive promoter for <i>Aspergillus niger</i>.
		+
		+	===Characterization===
		+	<html>
		+	This is a synthetic constitutive promoter, created as part of the LEAP (Library of Engineered Aspergillus Promoters) project. It is based on an unknown promoter from different <i>Aspergillus</i> spp., and the gene was chosen based on RNA-seq data from <i>Aspergillus niger</i>. [1] This version is a consensus sequence of the An07g08210 promoters in <i>Aspergillus</i> and is expected to have a weak constitutive expression.
		+	<br><br>
		+	This promoter was characterised using an mCherry test device,<a href=”https://parts.igem.org/wiki/index.php?title=Part:BBa_K3046009” target=”_blank”>BBa_K3046009</a>, inserted into an AMA1-based test plasmid, <a href=”https://parts.igem.org/wiki/index.php?title=Part:BBa_K3046021” target=”_blank_”>BBa_K3046021</a>, and characterisation was done a microbioreactor (BioLector, m2p-labs) <br>
		+	The microtiter scale cultures were made by inoculating 10<sup>7</sup> spores in 1.5 mL minimal media, and cultures were grown at 30 °C with mixing at 1000 rpm for 78 hours. Both biomass (measured in light scattering units) and fluorescence (at Ex/Emi wavelengths 580 nm/625 nm) was measured continuously.
		+	<br>
		+	The predicted behavior of this promoter, is described by the model, which is summarized by the figure below. PLEAPunk_1 is expected to show constitutive expression with medium promoter strength.
		+	<br>
		+	<br>
		+	<img src="https://2019.igem.org/wiki/images/thumb/3/37/T--DTU-Denmark--AN07pngRNA.png/650px-T--DTU-Denmark--AN07pngRNA.png" style="width: 80%; padding: 15px;" >
		+	<figure>
		+	<figcaption> Figure 1: The figure shows RNA-seq data for <i>Aspergillus niger</i> in both exponential and stationary phase with the unk gene marked in red. The x-axis is the promoter activity in the stationary phase and the y-axis is the promoter activity in the exponential phase, both axes are depicted on a log scale. Here we see that the promoter should be relatively constitutive with a high expression.
		+
		+
		+	</figcaption>
		+	</figure>
		+
		+	<br>
		+	For the microtiter scale, the promoter was evaluated in a biolector, producing the following results with regards to growth, fluorescence and dynamic promoter activity.
		+	<br>
		+	<img src="https://static.igem.org/mediawiki/parts/3/3e/T--DTU-Denmark--unk1promodynamics.png" style="width: 60%; padding: 15px;" >
		+	<figure>
		+	<figcaption> Figure 2: When analyzed in the microtiter scale on a biolector, the red fluorescence and biomass has been measured and the Dynamic Promoter Activity has been calculated. On the graph Dynamic Promoter Activity (DPA) is green, the biomass is measured in Light Scattering Units (LSU) is in blue, and red fluorescence (RFP) is shown in red. The graphs have been normalized for LSU.
		+	Here it is seen that the promoter has a low dynamic promoter activity that firsts begins to rise at 60 hours.
		+	</figcaption>
		+	</figure>
		+	</html>
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Latest revision as of 03:19, 14 December 2019

PLEAPunk_1

This is a synthetic constitutive promoter, created as part of the LEAP (Library of Engineered Aspergillus Promoters) project

Usage and Biology

This is a weak constitutive promoter for Aspergillus niger.

Characterization

This is a synthetic constitutive promoter, created as part of the LEAP (Library of Engineered Aspergillus Promoters) project. It is based on an unknown promoter from different Aspergillus spp., and the gene was chosen based on RNA-seq data from Aspergillus niger. [1] This version is a consensus sequence of the An07g08210 promoters in Aspergillus and is expected to have a weak constitutive expression.

This promoter was characterised using an mCherry test device,BBa_K3046009, inserted into an AMA1-based test plasmid, BBa_K3046021, and characterisation was done a microbioreactor (BioLector, m2p-labs)
The microtiter scale cultures were made by inoculating 10⁷ spores in 1.5 mL minimal media, and cultures were grown at 30 °C with mixing at 1000 rpm for 78 hours. Both biomass (measured in light scattering units) and fluorescence (at Ex/Emi wavelengths 580 nm/625 nm) was measured continuously.
The predicted behavior of this promoter, is described by the model, which is summarized by the figure below. PLEAPunk_1 is expected to show constitutive expression with medium promoter strength.

For the microtiter scale, the promoter was evaluated in a biolector, producing the following results with regards to growth, fluorescence and dynamic promoter activity.

Sequence and Features