Part:BBa_K1371041

RFP-DEBS1

DEBS1 was fused with red fluorescent protein

Sequence and Features

Fluorescence detection analyses

To further confirm the expression of DEBS1, we monitored the fluorescence of RFP under Zeiss LSM710 confocal microscope (Fig.1). The results showed that after excitation with lazer source, red fluorescence was monitored in the RFP+DEBS1+TE transformant, while in the BL21 strain, no fluorescence was detected. These results indicate that RFP+DEBS1+TE was successfully expressed in the transformant.

RT-PCR validation on transcriptional level

We used RT-PCR to examine the expression of the target genes on transcriptional level. We used 16S rRNA gene as an house keeping gene to compare the expression level of target genes. The results showed that DEBS1 gene was successfully expressed, albeit the transcription level was relatively low compared with other target genes (acc, pcc and sfp) whose transcription are controlled by T7 promoter as well.

UPLC-MS/MS Detection of TKL 1B

To test if RFP+DEBS1+TE was functionally expressed, the transformant was grown in Luria Broth (LB) liquid medium and induced with IPTG. After 48h of induction, cells were harvested and the supernatant was used for the extraction of the product TKL1B. After extraction, the samples were concentrated by 5 times and subjected into a triple quadrupole mass spectrometry and monitored under an MRM mode using the parent ion /product ion=173.1/155.1 channel. The retention time of the target product in the UPLC column was 6.42 min, using water/methanol gradient elution protocol. We monitored a strong response at m/z = 155.1 ion pair in the RFP+DEBS1+TE transformant sample. The ion pair of 173.1/155.1 is specific to the expected product TKL1B, and is in consistent with previous studies. These results demonstrated that TKL1B was successfully produced from the transformant.^[4]