Revision as of 04:00, 15 August 2023 (view source) Registry (Talk | contribs)		Latest revision as of 00:54, 11 October 2023 (view source) Bobbbb (Talk | contribs)
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	<partinfo>BBa_K4887006 short</partinfo>		<partinfo>BBa_K4887006 short</partinfo>
−	Hygromycin resistance gene.	+	It is a hygromycin resistance gene.
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	<partinfo>BBa_K4887006 SequenceAndFeatures</partinfo>		<partinfo>BBa_K4887006 SequenceAndFeatures</partinfo>
		+	<html>
		+	<style>
		+	li {
		+	list-style-type: none;
		+	padding: 0;
		+	}
		+	.bild{
		+	max-width: 70%;
		+	max-height: auto;
		+	}
		+	.red{
		+	color:red;
		+	}
		+	.center {
		+	display: flex;
		+	justify-content: center;
		+	align-items: center;
		+	flex-direction: column;
		+	height: 60vh; /*注: 通过更改该数值可以减少 图片及配文 和 图片下面内容的间距 但是不能太小（>40）*/
		+	}
		+
		+	.unterschrift {
		+	text-align: center;
		+	}
		+	#toobig{
		+	max-width:30%;
		+	}
		+
		+	</style>
		+
		+	<h1>6.5 Results:</h1>
		+	<h2>(1) Selection of postively transformed calli with hygromycin</h2>
		+	When enough of sweet potato embryogenic callus ware obtained, they were infected with the A. tumefaciens transformants containing the vector for CRISPR-knockout expression by co-culture <b class="red">(Fig. 1A)</b>. After selection with hygromycin, positive transformed calli were obtained <b class="red">(Fig. 1B)</b>.
		+
		+	<div class="center">
		+	<img class="bild toobig" src="https://static.igem.wiki/teams/4887/wiki/images/images/part-embryogenic-callus-co-culture-with-a-tumefaciens-transformants.png" />
		+	<div class="unterschrift">
		+	<b>
		+	Fig. 11 Embryogenic callus co-culture with A. tumefaciens transformants (A) and selection of postively transformed calli with hygromycin (B)
		+	</b>
		+	</div>
		+	</div>
		+
		+
		+	<h2>(2) PCR detection for gene HygR.</h2>
		+	Genome DNA of the transgenic lines was extracted from leaves of these two regenerated seedlings. PCR detection on the genomes was performed by using primers designed based on the HygR protein gene. As the result, the transgenic lines 23216004 and 23216005 were further validated <b class="red">(Fig. 2)</b>.
		+	The sequences of the primers were as bellow:
		+	<ul>
		+	<li>HygR-F: 5’-Atgaaaaagcctgaactcac-3’</li>
		+	<li> HygR-R: 5’-ctatttctttgccctcggac-3’</li>
		+	</ul>
		+
		+	<div class="center">
		+	<img class="bild" src="https://static.igem.wiki/teams/4887/wiki/images/images/part-detection-results-of-pcrs-for-gene-hygr.png" />
		+	<div class="unterschrift">
		+	<b>
		+	Fig. 2 Detection results of PCR for gene HygR.
		+	</b>
		+	</div>
		+	</div>
		+	</html>
	<!-- Uncomment this to enable Functional Parameter display		<!-- Uncomment this to enable Functional Parameter display

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Latest revision as of 00:54, 11 October 2023

HygR

It is a hygromycin resistance gene.

Sequence and Features

6.5 Results:

(1) Selection of postively transformed calli with hygromycin

When enough of sweet potato embryogenic callus ware obtained, they were infected with the A. tumefaciens transformants containing the vector for CRISPR-knockout expression by co-culture (Fig. 1A). After selection with hygromycin, positive transformed calli were obtained (Fig. 1B).

(2) PCR detection for gene HygR.

Genome DNA of the transgenic lines was extracted from leaves of these two regenerated seedlings. PCR detection on the genomes was performed by using primers designed based on the HygR protein gene. As the result, the transgenic lines 23216004 and 23216005 were further validated (Fig. 2). The sequences of the primers were as bellow:

• HygR-F: 5’-Atgaaaaagcctgaactcac-3’
• HygR-R: 5’-ctatttctttgccctcggac-3’