Difference between revisions of "Team:Hong Kong-CUHK/methods"

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<h1><b><u>The construction of the MFO</u></b></h1>
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<h1><b>Construction of Magnetosome Forming Operon</b></h1>
  
  
<p><font face="Times New Roman" size="4pt">Our first construct is called the MFO, which stands for the magnetosome forming operon. Different operons that are used to produce and regulate the magnetosome formation[1]. Among them, it is the <i>mamAB</i> operon that is the crucial operon that is needed for the production of magnetosome. Other operons like <i>mamGFDC</i>, <i>mamXY</i>, <i>mms6</i> et cetera are more frequently used for regulating the size and shape and the biominerlization that facilitate the formation of magnetosome[2].<br>
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<p>Our first construct is called Magnetosome Forming Operon (MFO). Different operons are involved in regulation of magnetosome formation[1]. Among them, it is the <i>mamAB</i> operon essential for magnetosome production. Other operons like <i>mamGFDC</i>, <i>mamXY</i> and <i>mms6</i> regulate size and shape of magnetite, and the biominerlization to facilitate the formation of magnetosome [2].<br>
  
Therefore, we would only insert the <i>mamAB</i> operon from <i> Magnetospirillum gryphiswaldense </i> (MSG) to bacteria <i>Azotobacter Vinelandii</i>, hoping to use minimal number of genes to produce functional magnetosome. Future insight is given to make the magnetosome formation progress easier. <br>
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Therefore, we would only insert the <i>mamAB</i> operon from <i> Magnetospirillum gryphiswaldense </i> (MSG) to bacteria <i>Azotobacter vinelandii</i>, hoping to use minimal number of genes to produce functional magnetosomes. Future insight is given to make the magnetosome formation progress easier. <br>
  
Considering the rather large size of <i>mamAB</i> operon, which is 16.4 KB, a new method was employed to help its transfer into the <i>Azotobacter vinelandii</i>. The overview of <i>mamAB</i> construct cloning strategy is shown in Figure 1.  
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Considering the rather large size of <i>mamAB</i> operon, which is 16.4 kb, a new method was employed to help its transfer into the <i>Azotobacter vinelandii</i>. The overview of <i>mamAB</i> construct cloning strategy is shown in Figure 1.  
  
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<h1><b><u>The insertion kit:</u></b></h1>
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<h1><b>The insertion Kit</b></h1>
 
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<p><font face="Times New Roman" size="4pt">This construct consists of a <i>mamC</i> gene, a gene coding for a trans-membrane protein [3] on the magnetosome membrane. Unlike usual recombinant methods in which insert is put between the multiple restriction sites, we are putting our <i>mamC</i> gene in front of them. Thus it enables the attachment of any protein desired to the magnetosome membrane, through insertion into the multiple restriction sites fusing with mamC. (For your interest, this is done by removing the stop codon of the mamC gene and the start codon of the desired protein, for example an antibody, making it a mamC fused protein).<br>
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<p>This construct consists of a <i>mamC</i> gene, a gene coding for a transmembrane protein [3] on the magnetosome membrane. Unlike usual recombinant methods in which insert is put between the multiple restriction sites, we are putting our <i>mamC</i> gene in front of them. Thus it enables the attachment of any protein desired to the magnetosome membrane, through insertion into the multiple restriction sites fusing with mamC. (For your interest, this is done by removing the stop codon of the mamC gene and the start codon of the desired protein, for example an antibody, making it a mamC fused protein).<br>
 
<br>
 
<br>
Normal method of inserting the gene of interest by restriction digestion and ligation is not possible in here. Instead, the whole plasmid has to be synthesized by ourselves using PCR method. The overview of cloing strategy is summarized in Figure 2. Four fragments would be produced firstly: B0015 – the double terminator; backbone with kanamycin; J13002 (which consists of the constitutive promoter R0040 and the RBS); and <i>mamC</i>.<br>
+
Normal method of inserting the gene of interest by restriction digestion and ligation is not possible in here. Instead, the whole plasmid has to be synthesized by ourselves using PCR method. The overview of cloning strategy is summarized in Figure 2. Four fragments would be produced firstly: B0015 – the double terminator; backbone with kanamycin; J13002 (which consists of the constitutive promoter R0040 and the RBS); and <i>mamC</i>.<br>
  
 
Through the over-lapping PCR of these four fragments, one linear fragment would be produced. And we have designed PstI sites at both the start and the end of the fragment. Consequently, by cutting the PstI site and ligate it, a circular plasmid will be produced. </p></font><br>
 
Through the over-lapping PCR of these four fragments, one linear fragment would be produced. And we have designed PstI sites at both the start and the end of the fragment. Consequently, by cutting the PstI site and ligate it, a circular plasmid will be produced. </p></font><br>

Revision as of 19:08, 18 September 2015

Construction of Magnetosome Forming Operon

Our first construct is called Magnetosome Forming Operon (MFO). Different operons are involved in regulation of magnetosome formation[1]. Among them, it is the mamAB operon essential for magnetosome production. Other operons like mamGFDC, mamXY and mms6 regulate size and shape of magnetite, and the biominerlization to facilitate the formation of magnetosome [2].
Therefore, we would only insert the mamAB operon from Magnetospirillum gryphiswaldense (MSG) to bacteria Azotobacter vinelandii, hoping to use minimal number of genes to produce functional magnetosomes. Future insight is given to make the magnetosome formation progress easier.
Considering the rather large size of mamAB operon, which is 16.4 kb, a new method was employed to help its transfer into the Azotobacter vinelandii. The overview of mamAB construct cloning strategy is shown in Figure 1.

Figure 3: Cloning strategy for mamAB operon

The insertion Kit


This construct consists of a mamC gene, a gene coding for a transmembrane protein [3] on the magnetosome membrane. Unlike usual recombinant methods in which insert is put between the multiple restriction sites, we are putting our mamC gene in front of them. Thus it enables the attachment of any protein desired to the magnetosome membrane, through insertion into the multiple restriction sites fusing with mamC. (For your interest, this is done by removing the stop codon of the mamC gene and the start codon of the desired protein, for example an antibody, making it a mamC fused protein).

Normal method of inserting the gene of interest by restriction digestion and ligation is not possible in here. Instead, the whole plasmid has to be synthesized by ourselves using PCR method. The overview of cloning strategy is summarized in Figure 2. Four fragments would be produced firstly: B0015 – the double terminator; backbone with kanamycin; J13002 (which consists of the constitutive promoter R0040 and the RBS); and mamC.
Through the over-lapping PCR of these four fragments, one linear fragment would be produced. And we have designed PstI sites at both the start and the end of the fragment. Consequently, by cutting the PstI site and ligate it, a circular plasmid will be produced.


Figure 4: Pstl ligation




[1]. LOHßE, Anna, et al. Genetic dissection of the mamAB and mms6 operons reveals a gene set essential for magnetosome biogenesis in Magnetospirillum gryphiswaldense. Journal of bacteriology, 2014, 196.14: 2658-2669.

[2]. CHEN, Zhucheng; YANG, Haijuan; PAVLETICH, Nikola P. Mechanism of homologous recombination from the RecA–ssDNA/dsDNA structures. Nature, 2008, 453.7194: 489-494.

[3]. XU, Jun, et al. Surface expression of protein A on magnetosomes and capture of pathogenic bacteria by magnetosome/antibody complexes. Frontiers in microbiology, 2014, 5.