Ent MedChemExpress DprE1-IN-2 protein (YFP) as an acceptor fluorescent protein. It is known that the S208F/V224L mutant of GFP has a weak propensity to form a homo-dimer [20] while the A206K mutant exists as a stable monomer [21]. We introduced A206K and S208F/V224L mutations into CFP (termed mCFP and dCFP, respectively) and into YFP (termed mYFP and dYFP, respectively). They were connected to ODNs and assembled into multi-proteinDNA complexes in such a way that mCFP and mYFP (or dCFP and dYFP) were placed either at adjacent positions or at opposite ends. The fluorescence spectrum was measured and the ratio of fluorescent intensity of 520 nm/480 nm was calculated as an indicator of FRET from CFP to YFP (Fig. 4). As a control, the DNA backbone between CFP and YFP was cleaved by restriction enzyme EcoRI so that they could freely diffuse in the medium. When mCFP and mYFP were aligned in adjacent positions, the ratio of 520 nm/480 nm was decreased by EcoRI treatment, reflecting their physical vicinity in the multi-protein-DNA complex (Fig. 4A). No spectral change occurred before and after EcoRI treatment in the case where mCFP and mYFP were placed at opposite ends, indicating they are distant enough to abolish FRET. Combination of dCFP and dYFP, on the contrary, induced FRET even when they were placed at the end positions (Fig. 4B). The interaction between dCFP and dYFP is so weak that FRET disappeared once the DNA backbone was lost by EcoRI treatment. Obviously, increased local concentrations of dCFP and dYFP and flexibility of the hinge regions of the DNA backbone facilitate dimer formation with weak interactions.DiscussionThe multi-protein-DNA complex reported here enables nanoscale alignment of several different proteins along a DNA backbone. Importantly, proteins are not tightly immobilized. Rather, they have some freedom of motion and can find the best orientation to interact with each other. Effective local concentrations of proteins are estimated to be ,4.2 mM when six proteins are aligned in a DNA backbone and ,1.4 mM when two proteins are aligned at positions on opposite ends (calculated from radius of gyration of freely-jointed chain model). These very high concentrations enable association of proteins with very weak association force. The nano-scale, flexible protein alignment has large potential for basic and application studies. Reaction cycles of multi-subunit complexes containing steps of subunit dissociation/ association can occur more easily in the multi-protein-DNA complex.Supporting InformationFigure S1 Mass spectroscopy analysis of the synthesized MedChemExpress Licochalcone-A N3-ODN (A) 59-aimino-ODN(No. 5) (17033Da) was detected as a peak at 17030.55 m/z. (B) The synthesized N3ODN(No. 5) (17306 Da) was detected as a peak at 17308.29 m/z. (C) Mass spectrum of the equal molar mixture of 59-aimino-ODN and N3-ODN. The peaks of 59-aimino-ODN (17033.28 m/z) and N3-ODN (17307.31 m/z) were indicated. (TIF) Figure S2 Conjugation reaction of sfGFP and ODN was carried out using His6-sfGFP (without extra cysteine) and His6-sfGFP-Cys (with an extra cysteine) in the presence or 11967625 absence of DBCO-PEG4-maleimide andFlexible Alignment of ProteinN3-ODN. The conjugated product was observed only for His6sfGPF-Cys+DBCO-PEG4-maleimide+N3-ODN. (TIF)Figure S3 Mass spectroscopy analysis of sfGFP-ODN. (A) His6-sfGFP-Cys (27758Da) was detected as a peak at 27730.40 m/z. (B) His6-sfGFP-ODN (No. 5) (45739 Da) was detected as a peak at 45859.31 m/z. (TIF)(S1) and right panels (S2) of Fig. 3. Scan area, 8.Ent protein (YFP) as an acceptor fluorescent protein. It is known that the S208F/V224L mutant of GFP has a weak propensity to form a homo-dimer [20] while the A206K mutant exists as a stable monomer [21]. We introduced A206K and S208F/V224L mutations into CFP (termed mCFP and dCFP, respectively) and into YFP (termed mYFP and dYFP, respectively). They were connected to ODNs and assembled into multi-proteinDNA complexes in such a way that mCFP and mYFP (or dCFP and dYFP) were placed either at adjacent positions or at opposite ends. The fluorescence spectrum was measured and the ratio of fluorescent intensity of 520 nm/480 nm was calculated as an indicator of FRET from CFP to YFP (Fig. 4). As a control, the DNA backbone between CFP and YFP was cleaved by restriction enzyme EcoRI so that they could freely diffuse in the medium. When mCFP and mYFP were aligned in adjacent positions, the ratio of 520 nm/480 nm was decreased by EcoRI treatment, reflecting their physical vicinity in the multi-protein-DNA complex (Fig. 4A). No spectral change occurred before and after EcoRI treatment in the case where mCFP and mYFP were placed at opposite ends, indicating they are distant enough to abolish FRET. Combination of dCFP and dYFP, on the contrary, induced FRET even when they were placed at the end positions (Fig. 4B). The interaction between dCFP and dYFP is so weak that FRET disappeared once the DNA backbone was lost by EcoRI treatment. Obviously, increased local concentrations of dCFP and dYFP and flexibility of the hinge regions of the DNA backbone facilitate dimer formation with weak interactions.DiscussionThe multi-protein-DNA complex reported here enables nanoscale alignment of several different proteins along a DNA backbone. Importantly, proteins are not tightly immobilized. Rather, they have some freedom of motion and can find the best orientation to interact with each other. Effective local concentrations of proteins are estimated to be ,4.2 mM when six proteins are aligned in a DNA backbone and ,1.4 mM when two proteins are aligned at positions on opposite ends (calculated from radius of gyration of freely-jointed chain model). These very high concentrations enable association of proteins with very weak association force. The nano-scale, flexible protein alignment has large potential for basic and application studies. Reaction cycles of multi-subunit complexes containing steps of subunit dissociation/ association can occur more easily in the multi-protein-DNA complex.Supporting InformationFigure S1 Mass spectroscopy analysis of the synthesized N3-ODN (A) 59-aimino-ODN(No. 5) (17033Da) was detected as a peak at 17030.55 m/z. (B) The synthesized N3ODN(No. 5) (17306 Da) was detected as a peak at 17308.29 m/z. (C) Mass spectrum of the equal molar mixture of 59-aimino-ODN and N3-ODN. The peaks of 59-aimino-ODN (17033.28 m/z) and N3-ODN (17307.31 m/z) were indicated. (TIF) Figure S2 Conjugation reaction of sfGFP and ODN was carried out using His6-sfGFP (without extra cysteine) and His6-sfGFP-Cys (with an extra cysteine) in the presence or 11967625 absence of DBCO-PEG4-maleimide andFlexible Alignment of ProteinN3-ODN. The conjugated product was observed only for His6sfGPF-Cys+DBCO-PEG4-maleimide+N3-ODN. (TIF)Figure S3 Mass spectroscopy analysis of sfGFP-ODN. (A) His6-sfGFP-Cys (27758Da) was detected as a peak at 27730.40 m/z. (B) His6-sfGFP-ODN (No. 5) (45739 Da) was detected as a peak at 45859.31 m/z. (TIF)(S1) and right panels (S2) of Fig. 3. Scan area, 8.