Plasmid construction and validation

We first amplified the glnK promoter and nifH promoter from the genome of Sinorhizobium fredii CCBAU45436, amplified gfp and designed sgRNAs from pRJPaph-bjGFP plasmid, and ligated them using overlap PCR. To verify the effect of the regulation module alone, we connected it with the nuoA promoter-Cas12k and the linearized pBBR1MCS-2 (Figure 2-2-1). The recombinant plasmid was transformed into E. coli (DH5α).

Triparental mating and validation

The verified correct colonies were inoculated into kanamycin-resistant LB liquid medium under shaking condition. Then we conducted triparental mating using the correct colony we obtained above, Helper and Sinorhizobium fredii CCBAU45436. Then colony PCR was performed on colonies grown on TY/NA/Kan solid medium incubated at 28°C for 24 h using the universal primer M13F/R.

Fluorescence intensity verification

We utilized its fluorescence expression intensity to verify whether the regulation module functioned properly. We set up four sets of experiment with high nitrogen and high oxygen, low nitrogen and high oxygen, high nitrogen and low oxygen, as well as low nitrogen and low oxygen for verification. Subsequently, we used M9 medium without nitrogen source, then added different concentrations of ammonium chloride to form nitrogen concentration gradient. We added petroleum jelly after boiling the medium to isolate medium against atmosphere, creating anaerobic conditions. The OD600 value of the bacterial solution was determined after a period of shaking and incubation, and the fluorescence intensity of the bacterial solution was determined using a fluorescence spectrophotometer (Figure 2-4-1 and Figure 2-4-2).