Difference between revisions of "Part:BBa K2912015"

Revision as of 00:50, 17 October 2019

Trp_Lysis gene

Trp_Lysis gene expression can be controlled by the concentration of Tryptophan

Sequence and Features

Assembly Compatibility:

10
COMPATIBLE WITH RFC[10]
12
INCOMPATIBLE WITH RFC[12]
Illegal NheI site found at 7
Illegal NheI site found at 30
21
COMPATIBLE WITH RFC[21]
23
COMPATIBLE WITH RFC[23]
25
COMPATIBLE WITH RFC[25]
1000
COMPATIBLE WITH RFC[1000]

Usage and Biology

The lysis gene from colicin-producing strains of bacteria encodes the lysis protein which can cause the host cell to lyze as long as the protein is activated. On the basic of its biological function, we can use lysis gene to break our engineering E.coli and release the interior cell contents when it's time to extract our product-shRNA by adding a Tryptophan attenuator between a RBS and lysis gene

We transformed the expression vector into HT115 (DE3) E.coli by heat-shock method, and they were cultured in 1 LB liquid medium to exact exponential phase. Afterwards, we started a cell growth curve experiment of our engineering E.coli(illustrated with Fig.1)

Revision as of 17:59, 15 October 2019 (view source) EmrysTang (Talk \| contribs) (→‎Usage and Biology) ← Older edit		Revision as of 00:50, 17 October 2019 (view source) Mackintosh (Talk \| contribs) (→‎Usage and Biology) Newer edit →
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	The lysis gene from colicin-producing strains of bacteria encodes the lysis protein which can cause the host cell to lyze as long as the protein is activated. On the basic of its biological function, we can use lysis gene to break our engineering E.coli and release the interior cell contents when it's time to extract our product-shRNA by adding a Tryptophan attenuator between a RBS and lysis gene		The lysis gene from colicin-producing strains of bacteria encodes the lysis protein which can cause the host cell to lyze as long as the protein is activated. On the basic of its biological function, we can use lysis gene to break our engineering E.coli and release the interior cell contents when it's time to extract our product-shRNA by adding a Tryptophan attenuator between a RBS and lysis gene

−	We transformed the expression vector into HT115 (DE3) E.coli by heat-shock method	+	We transformed the expression vector into HT115 (DE3) E.coli by heat-shock method, and they were cultured in 1 LB liquid medium to exact exponential phase. Afterwards, we started a cell growth curve experiment of our engineering E.coli(illustrated with Fig.1)