Composite
SV40-4-2

Part:BBa_K2446034

Designed by: Yijie Pan   Group: iGEM17_Fudan   (2017-10-21)


SV40_4_PIP promoter

This part (Sv40 4*PIP ) is a mammalian synthetic promoter (SynPro) based on Sv40 promoter (BBa_K2446052) and four repeats of PIP binding sites . We inset the 4*PIP binding sites behind the Sv40 promoter. Sv40 promoter is a constitutive expression promoter from the simian vacuolating virus 40. In this way, we can use our mammalian synthetic transcription factors (SynTFs) which is a fusing protein PIP_DBD_(G4S) linker_NLS_KRAB. The PIP-DBD can bind to the 4*PIP binding sites specifically[1] and the KRAB domain can repress the expression of Sv40 4*PIP promoter [2]. The corresponding SynTF of Sv40-4_PIP is ZF_PIP_KRAB (BBa_K2446038).

Figure 1: The design of SynTF-SynPros.

Figure 1: The design of SynTF-SynPros.

The information of other SynTF-SynPros is showed in the table below.

SynTFs SynPros
Gal4-KRAB(TF-KRAB-1) BBa_K2446037 Sv40-UAS(Sv40-UAS) BBa_K2446036
ZF_PIP_KRAB(TF-KRAB-2) BBa_K2446045 SV40_2/4/8_PIP BBa_K2446033/BBa_K2446034/BBa_K2446035
ZF_21-16KRAB(TF-KRAB-3) BBa_K2446039 SV40_8_ZF_21-16 BBa_K2446030
ZF_42-10_KRAB(TF-KRAB-4) BBa_K2446040 SV40_8_ZF_42-10 BBa_K2446025
ZF_43-8_KRAB(TF-KRAB-5) BBa_K2446041 SV40_2/4/8_ZF_43-8 BBa_K2446026/BBa_K2446027/BBa_K2446028
ZF_54-8_KRAB(TF-KRAB-6) BBa_K2446042 SV40_8_ZF_54-8 BBa_K2446029
ZFHD1_KRAB(TF-KRAB-7) BBa_K2446043 SV40_4_ZFHD1 BBa_K2446032


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]


Experiments

SynTF-SynPro Pairs

Figure 2: the testing circuits of PIP-KRAB& Sv40_4_PIP pair

Figure 2: the testing circuits of PIP-KRAB& Sv40_4_PIP pair

To make sure the SynTF-SynPro pairs work in mammalian cells, we use the circuits above to test if the PIP-KRAB can repress the expression of Sv40_4_PIP indeed. PIP-KRAB is linked to the C terminal of EGFP by the link of P2A. And mCherry expressions is controlled by corresponding SynPro (Sv40_4_PIP). These circuits are both inserted in to the mammalian expression vactor pML2. We transfect pML2-Sv40_4_PIP into Hela cells and measure the fluorescence intensity of mCherry by flow cytometer to get the basic expression intensity of Sv40_4_PIP. We also co-transfect the pML2-PIP-KRAB with pML2-Sv40_4_PIP into Hela cells at the same time. Then measure the fluorescence intensity of mCherry again to get the expression intensity of Sv40_4_PIP influenced by PIP-KRAB. The results of the experiment is showed below. The SynTF PIP can silence the expression of the SynPro Sv404_PIP in 43 folds.

Figure 3:The results of PIP-KRAB&SV40_4_PIP testing: (A) The red points is the cells before co-transfecting PIP-KRAB and the blue points is the cells after co-transfecting PIP-KRAB. It’s easy to see that the red points depart from the diagonal and higher than the blue points. So the expression of mCherry silenced after the expression of PIP-KRAB;(B) The red area is the fluorescence intensity of mCherry before co-transfecting PIP-KRAB and the blue area is the intensity after co-transfecting PIP-KRAB.(C) The statistical result of all of the SynTFs-SynPros pairs: PIP-KRAB can silence the expression intensity of Sv40_4_PIP in 43 folds

Figure 3: The results of PIP-KRAB&SV40_4_PIP testing: (A) The red points is the cells before co-transfecting PIP-KRAB and the blue points is the cells after co-transfecting PIP-KRAB. It’s easy to see that the red points depart from the diagonal and higher than the blue points. So the expression of mCherry silenced after the expression of PIP-KRAB;(B) The red area is the fluorescence intensity of mCherry before co-transfecting PIP-KRAB and the blue area is the intensity after co-transfecting PIP-KRAB. (C) The statistical result of all of the SynTFs-SynPros pairs: PIP-KRAB can silence the expression intensity of Sv40_4_PIP in 43 folds

SynTF-SynPro Orthogonality

To construct our [http://2017.igem.org/Team:Fudan/Model/GTN| Strip module], more than one SynTF-SynPro pairs would be applied. Thus, the interaction between the pairs would influence or ruin our construction. We did massive orthogonality experiments to avoid that. We observed all of the 5 pairs were actually orthogonal, as you could see the grids on the diagonal were always the darkest. The three DBDs commonly used in previous works were didn’t let us down. However, the expression level of these RE loaded SynPros were relative low compared to SynPro(S)-ZF serials. As the blue rectangle in the lower right corner of the orthogonality may showed the SynPro(S)-ZF has high basic expression with unpaired SynTFs, but could be silenced to the similar fold of commonly used DBDs corresponding SynPros. The SynPro(S)-ZF was likely won’t be target by other unpaired DBD, hence the purple appeared on the bottom rows.

Figure 4: the SynTF-SynPro pairs’ Orthogonality. Grids in blue rectangle showed that SynTF-SynPro pairs constructed by using SynZF as DBD with well orthogonality. Grids in pink rectangles replaced our favorite SynTF-SynPro pairs. At least 20,000 cells were analyzed for each condition in both histogram and each grid in heat map. Data are recorded by FACS at 24h after cotransfecting.

Figure 4: the SynTF-SynPro pairs’ Orthogonality. Grids in blue rectangle showed that SynTF-SynPro pairs constructed by using SynZF as DBD with well orthogonality. Grids in pink rectangles replaced our favorite SynTF-SynPro pairs. At least 20,000 cells were analyzed for each condition in both histogram and each grid in heat map. Data are recorded by FACS at 24h after cotransfecting.

References

[1] M. Fussenegger et al., Streptogramin-based gene regulation systems for mammalian cells. Nature biotechnology 18, 1203--1208 (2000).

[2] R. Witzgall, E. O'Leary, A. Leaf, D. Onaldi, J. V. Bonventre, The Krüppel-associated box-A (KRAB-A) domain of zinc finger proteins mediates transcriptional repression. Proceedings of the National Academy of Sciences 91, 4514-4518 (1994).
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