Difference between revisions of "Part:BBa K2916016"

Revision as of 19:22, 21 October 2019

Expression of AsnRS in E.coli

This part is used for expression of Asparaginyl-tRNA synthetase needed for the PURE and OnePot PURE cell-free systems.

Usage and Biology

Used in OnePot PURE

Characterization

Expression and purification of AsnRS

AsnRS is one of the proteins we used for the OnePot PURE cell-free system. We expressed it in M15 E.coli strain using a pQE30 vector. The expression system has a T5 lac operator, RBS and a lambda t0 Terminator, enabling us to regulate the expression with IPTG.

Methods

AsnRS was purified using our protocol . To test if the protein was actually expressed, we performed a SDS-PAGE that is presented below. On the left side we can see the results included in the initial OnePot PURE paper (Lavickova et al, 2019) while on the right (batch1_a,b and batch2_a,b) are the solutions we produced ourselves. (The procedure we followed and the conditions of the experiment can be found here).

control — **Figure 1:** SDS-PAGE of OnePot PURE protein solution.

Conclusion
AsnRS has a molecular weight of around 53kDa, but even though we cannot be absolutely sure if the band shown is only due to it, we may assume that it is expressed. To verify the existence and functionality of this protein we need to proceed with more experiments that would be mainly focused on the efficiency of the system.

OnePot PURE functionality test

To make sure that we have all the proteins in our OnePot PURE protein solution, and that they all function properly we need check if proteins can be expressed in our OnePot PURE cell-free system.

Methods

We expressed superfolding GFP following the protocol we designed in 10μl reactions, and measured the fluorescence on a plate reader at excitation wavelength of 535nm. We tested the expression using different concentrations of the sf GFP DNA template and also compared it with the fluorescence produced in PURExpress from NEB.

Conclusion
The expression was successful so we can confirm that AsnRS exists in our protein solution and is also functioning properly.

Sequence and Features

Assembly Compatibility:

10
COMPATIBLE WITH RFC[10]
12
INCOMPATIBLE WITH RFC[12]
Illegal NotI site found at 1119
21
COMPATIBLE WITH RFC[21]
23
COMPATIBLE WITH RFC[23]
25
COMPATIBLE WITH RFC[25]
1000
COMPATIBLE WITH RFC[1000]

@@ Line 4: / Line 4: @@
-This part is used for expression of Aspartate-tRNA synthetase needed for the PURE and OnePot PURE cell-free systems.
+This part is used for expression of Asparaginyl-tRNA synthetase needed for the PURE and OnePot PURE cell-free systems.
 <!-- Add more about the biology of this part here-->
@@ Line 11: / Line 11: @@
 Used in OnePot PURE
 ===Characterization===
-=='''Expression and purification of AspRS'''==
+=='''Expression and purification of AsnRS'''==
 <br/>
-AspRS is one of the proteins we used for the OnePot PURE cell-free system. We expressed it in M15 E.coli strain using a pQE30 vector. The expression system has a T5 lac operator, RBS and a lambda t0 Terminator, enabling us to regulate the expression with IPTG.<br/><br/>
+AsnRS is one of the proteins we used for the OnePot PURE cell-free system. We expressed it in M15 E.coli strain using a pQE30 vector. The expression system has a T5 lac operator, RBS and a lambda t0 Terminator, enabling us to regulate the expression with IPTG.<br/><br/>
 '''Methods'''
 <br/>
-AspRS was purified using our <html><a style="padding: 0px; margin: 0px;" href="https://www.protocols.io/view/protein-purification-for-onepot-pure-cell-free-sys-8auhsew"> protocol </a></html>. To test if the protein was actually expressed, we performed a SDS-PAGE that is presented below. On the left side we can see the results included in the initial OnePot PURE paper (<i>Lavickova et al, 2019</i>) while on the right (batch1_a,b and batch2_a,b) are the solutions we produced ourselves. (The procedure we followed and the conditions of the experiment can be found <html><a style="padding: 0px; margin: 0px;" href="https://www.protocols.io/view/sps-page-protein-electrophoresis-775hrq6"> here</a></html>).
+AsnRS was purified using our <html><a style="padding: 0px; margin: 0px;" href="https://www.protocols.io/view/protein-purification-for-onepot-pure-cell-free-sys-8auhsew"> protocol </a></html>. To test if the protein was actually expressed, we performed a SDS-PAGE that is presented below. On the left side we can see the results included in the initial OnePot PURE paper (<i>Lavickova et al, 2019</i>) while on the right (batch1_a,b and batch2_a,b) are the solutions we produced ourselves. (The procedure we followed and the conditions of the experiment can be found <html><a style="padding: 0px; margin: 0px;" href="https://www.protocols.io/view/sps-page-protein-electrophoresis-775hrq6"> here</a></html>).
 <br/>
@@ Line 34: / Line 35: @@
 '''Conclusion'''
-<br/> AspRS has a molecular weight of around 43kDa, so since we can see a band at that molecular weight level, we may assume that it is expressed. To verify the functionality of this protein we need to proceed with more experiments that would be mainly focused on the efficiency of the system.
+<br/> AsnRS has a molecular weight of around 53kDa, but even though we cannot be absolutely sure if the band shown is only due to it, we may assume that it is expressed. To verify the existence and functionality of this protein we need to proceed with more experiments that would be mainly focused on the efficiency of the system.
 <br/>
 <br/>
@@ Line 76: / Line 77: @@
 '''Conclusion'''
-<br/> The expression was successful so we can confirm that AspRS exists in our protein solution and is also functioning properly.
+<br/> The expression was successful so we can confirm that AsnRS exists in our protein solution and is also functioning properly.
 <br/>