Difference between revisions of "Part:BBa K1927002"
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die. By hydrolyzing the ring, it will make the molecule unable to bind to the cell wall | die. By hydrolyzing the ring, it will make the molecule unable to bind to the cell wall | ||
producing enzyme, thus the Penicillin have lost its destructive activity. | producing enzyme, thus the Penicillin have lost its destructive activity. | ||
− | + | ||
+ | ===Applications of BBa_K1927002=== | ||
+ | |||
+ | <p class="boxnotes leftext"><b>Generation of biobrick BBa_K1927002 and BBa_K1927003</b><br> | ||
+ | We wanted to calibrate our detection test with a biobrick of our own, in addition to the positive control (E. coli amp), negative control (E. coli without antibiotic resistance) and the purified protein from biobrick BBa_K1189031 as an additional positive control. </p> | ||
+ | |||
+ | <p class="boxnotes leftext"> | ||
+ | We retrieved the gene sequence for the Amp-gene from the standard E. coli vector pUC19 (http://www.snapgene.com/resources/plasmid_files/basic_cloning_vectors/pUC19/). The AmpR gene product is a β-lactamase class A which confers resistance to ampicillin, carbenicillin, and related antibiotics. The gene was designed to include prefix, suffix and start of vector sequence to make it ideal for Gibson assembly later on. Gene and primers was synthetized by IDT. We performed a Gibson assembly with the shipping vector pSB1C3 and our gene to generate biobrick BBa_K1927002. </p> | ||
+ | |||
+ | https://static.igem.org/mediawiki/2016/0/0c/T--UiOslo_Norway--plate002.jpg | ||
+ | <p class="boxnotes leftext imgcap"><i> | ||
+ | Figure 1: LB agar plate with chloramphenicol for growth of transformed <br> | ||
+ | bacteria(TOP10) with BBa_K1927002. The insert was inserted into the shipping <br> | ||
+ | vector pSB1C3 by Gibson assembly. </i></p> | ||
+ | |||
+ | |||
+ | https://static.igem.org/mediawiki/2016/1/14/T--UiOslo_Norway--pcr002.jpg | ||
+ | <p class="boxnotes leftext imgcap"><i> | ||
+ | Figure 2: Gel analysis of colony PCR with BBa_K1927002. <br> | ||
+ | The insert was inserted into the shipping vector pSB1C3 by using Gibson assembly. <br> | ||
+ | Lane 10 are DNA ladder (GeneRuler 1 kb DNA ladder, Thermo Fisher Scientific). <br> | ||
+ | Lane 11 are positive control (validated part BBa_K1927000). | ||
+ | <br> Lane 18-19 are different colonies from Gibson assembly. They show the appropriate <br> | ||
+ | band at approx. 1000bp.</i></p> | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
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Revision as of 12:32, 20 October 2016
β lactamase AmpR
This gene conveys resistance to a common antibiotic called Ampicillin. In research it is often used as a selection marker
Usage and Biology
During the last decade antibiotic resistance has grown not only in incidents but also in awareness among the public. Rapid detection of these incidents is essential in the battle against sophisticated bacteria. Beta lactamases are enzymes that provides one of the many mechanisms of antibiotic resistance. Its for this reason regulary used among researchers as a selection marker. Bacteria that has been subjected to a procedure where foreign DNA is introduced, an antibiotic resistance gene is often use to check if colonies succsesfully has taken up the DNA and expressed it.
An example of this is ampicillin which is a highly used selection marker. The need for a selection marker in genetical engineering has been shown extremly usefull. By transforming a bacteria with a particular gene plus an antibiotic resistance gene it allows the researcher to know exactly which colonies that has taken up the DNA. By plating them out on agar plates with a given antibiotic, only the bacteria with the resistance gene can grow. Cells that did not manage to take up the DNA will die.
The mechanism of beta lactamases are oriented to the bacterial cell wall. This cell wall is unique to bacteria and consist of several components. Gram Positive and gram negative bacteria will have a different cell wall composition. In general, Gram-positive bacteria have a thicker layer of cell wall as well as a layer of cytoplasmic membrane. These layers consist of several conserved compounds such as monomeric disaccharide tetrapeptide, which are usually also those that will trigger an immunological defence respons of the host. Gram-negative bacteria (e.g., Escherichia coli) typically contain an outer membrane, an intervening periplasmic space where a thin layer of cell wall resides, and a layer of cytoplasmic membrane. Beta lactamases are usually produced both by gram negative and positive bacteria, either from plasmid or chromosomally. Beta lactamases are able to resist several types of antibiotics. These antibiotics all have in common a 4 - atom ring called beta lactam ring which the enzyme are able to hydrolyze and break open and the molecule looses its antibacterial function.
Penicillin, a regulary used antibiotic have such a beta lactam ring. This drug was the first antibiotic to be discovered and is still widely used today. This ring will bind to an enzyme (DD –transpeptidase) that is in charge of renewing the bacterial cell wall. Without this enzyme there will be no new formations of peptidoglycans for the cell wall and the integrity of the bacterial cell wall will be lost, it will eventually rupture and the bacteria will die. By hydrolyzing the ring, it will make the molecule unable to bind to the cell wall producing enzyme, thus the Penicillin have lost its destructive activity.
Applications of BBa_K1927002
Generation of biobrick BBa_K1927002 and BBa_K1927003
We wanted to calibrate our detection test with a biobrick of our own, in addition to the positive control (E. coli amp), negative control (E. coli without antibiotic resistance) and the purified protein from biobrick BBa_K1189031 as an additional positive control.
We retrieved the gene sequence for the Amp-gene from the standard E. coli vector pUC19 (http://www.snapgene.com/resources/plasmid_files/basic_cloning_vectors/pUC19/). The AmpR gene product is a β-lactamase class A which confers resistance to ampicillin, carbenicillin, and related antibiotics. The gene was designed to include prefix, suffix and start of vector sequence to make it ideal for Gibson assembly later on. Gene and primers was synthetized by IDT. We performed a Gibson assembly with the shipping vector pSB1C3 and our gene to generate biobrick BBa_K1927002.
Figure 1: LB agar plate with chloramphenicol for growth of transformed
bacteria(TOP10) with BBa_K1927002. The insert was inserted into the shipping
vector pSB1C3 by Gibson assembly.
Figure 2: Gel analysis of colony PCR with BBa_K1927002.
The insert was inserted into the shipping vector pSB1C3 by using Gibson assembly.
Lane 10 are DNA ladder (GeneRuler 1 kb DNA ladder, Thermo Fisher Scientific).
Lane 11 are positive control (validated part BBa_K1927000).
Lane 18-19 are different colonies from Gibson assembly. They show the appropriate
band at approx. 1000bp.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI site found at 716