Not as easy as π: An insertional residue does not explain the π‐helix gain‐of‐function in two‐component FMN reductases

McFarlane, Jeffrey S.; Hagen, Richard; Chilton, Annemarie S.; Forbes, D.L.; Lamb, Audrey L.; Ellis, Holly R.

doi:10.1002/pro.3504

Cited by 6 publications

(7 citation statements)

References 33 publications

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“…The fluorescence decrease observed at higher pyridine nucleotide concentrations is due to unbound NADPH in solution . MsuE and the MsuD monooxygenase partner had a distinct specificity for FMN and NADPH in coupled assays with the MsuD monooxygenase partner, but the specificity of MsuE for each substrate in the absence of MsuD had not been determined . MsuE showed a similar affinity for FMN/FAD and NADH/NADPH, indicating there was no apparent preference for a specific substrate under equilibrium conditions (Figure C,D, Table , and Figure S1C,D).…”

Section: Resultsmentioning

confidence: 99%

“…The principal structural difference between the two groups of enzymes is the presence of a π-helix located at the dimer/dimer interface. 10,21,37,38 It has been proposed that the π-helix structure enables SsuE to transfer flavin through protein−protein interactions to the SsuD monooxygenase partner. [11][12][13]39 The SsuE−SsuD interaction sites are located at the dimer/dimer interface of SsuE so the enzyme would need to undergo a conformational change to form these interactions.…”

Section: Discussionmentioning

confidence: 99%

“…All reagents were purchased from Sigma-Aldrich, Biorad, or Fisher. The SsuE and MsuE genes were cloned separately into the RNA polymerase-dependent vector pET21a (Novagen) and expressed in Escherichia coli BL21 (DE3), as previously described. , The concentrations of SsuE and MsuE in solution were calculated with the molar extinction coefficient of each protein (20.3 and 7.4 mM –1 cm –1 ). , …”

Section: Methodsmentioning

confidence: 99%

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Oligomeric Changes Regulate Flavin Transfer in Two-Component FMN Reductases Involved in Sulfur Metabolism

Aloh,

Zeczycki,

Ellis

2023

Biochemistry

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The FMN reductases (SsuE and MsuE of the alkanesulfonate monooxygenase systems) supply reduced flavin to their partner monooxygenases for the desulfonation of alkanesulfonates. Flavin reductases that comprise two-component systems must be able to regulate both flavin reduction and transfer. One mechanism to control these distinct processes is through changes in the oligomeric state of the enzymes. Despite their similar overall structures, SsuE and MsuE showed clear differences in their oligomeric states in the presence of substrates. The oligomeric state of SsuE was converted from a tetramer to a dimer/tetramer equilibrium in the presence of FMN or NADPH in analytical ultracentrifugation studies. Conversely, MsuE shifted from a dimer to a single tetrameric state with FMN, and the NADPH substrate did not induce a similar oligomeric shift. There was a fast tetramer to dimer equilibrium shift occurring at the dimer/dimer interface in H/D-X investigations with apo SsuE. Formation of the SsuE/FMN complex slowed the tetramer/dimer conversion, leading to a slower exchange along the dimer/dimer interface. The oligomeric shift of the MsuE/FMN complex from a dimer to a distinct tetramer showed a decrease in H/D-X in the region around the π-helices at the dimer/dimer interface. Both SsuE and MsuE showed a comparable and significant increase in the melting temperature with the addition of FMN, indicating the conformers formed by each FMN-bound enzyme had increased stability. A mechanism that supports the different structural shifts is rationalized by the different roles these enzymes play in providing reduced flavin to single or multiple monooxygenase enzymes.

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Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Oligomeric Changes Regulate Flavin Transfer in Two-Component FMN Reductases Involved in Sulfur Metabolism

Aloh,

Zeczycki,

Ellis

2023

Biochemistry

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“…The concentrations of MsuD and MsuE proteins were determined from A 280 measurements using molar extinction coefficients of 49.4 and 7.54 mM −1 cm −1 , respectively. 17,18 Steady-State Kinetic Analyses. A coupled assay monitoring sulfite production was used to determine the steadystate kinetic parameters of SsuD and MsuD.…”

Section: Methodsmentioning

confidence: 99%

“…SsuD, SsuE, MsuD, and MsuE enzymes were purified as described previously. , The concentrations of SsuD and SsuE proteins were determined from A 280 measurements using molar extinction coefficients of 47.9 and 20.3 mM –1 cm –1 , respectively. The concentrations of MsuD and MsuE proteins were determined from A 280 measurements using molar extinction coefficients of 49.4 and 7.54 mM –1 cm –1 , respectively. , …”

Section: Methodsmentioning

confidence: 99%

Shorter Alkanesulfonate Carbon Chains Destabilize the Active Site Architecture of SsuD for Desulfonation

et al. 2022

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Bacteria have evolved to utilize alternative organosulfur sources when sulfur is limiting. The SsuE/SsuD and MsuE/MsuD enzymes expressed when sulfur sources are restricted, are responsible for providing specific bacteria with sulfur in the form of alkanesulfonates. In this study, we evaluated why two structurally and functionally similar FMNH2-dependent monooxygenase enzymes (MsuD and SsuD) are needed for the acquisition of alkanesulfonates in some bacteria. In desulfonation assays, MsuD was able to utilize the entire range of alkanesulfonates (C1–C10). However, SsuD was not able to utilize smaller alkanesulfonate substrates. Interestingly, SsuD had a similar binding affinity for methanesulfonate (MES) (15 ± 1 μM) as MsuD (12 ± 1 μM) even though SsuD was not able to catalyze the desulfonation of the MES substrate. SsuD and MsuD showed decreased proteolytic susceptibility in the presence of FMNH2 with MES and octanesulfonate (OCS). Tighter loop closure was observed for the MsuD/FMNH2 complex with MES and OCS compared to SsuD under comparable conditions. Analysis of the SsuD/FMNH2/MES structure using accelerated molecular dynamics simulations found three different conformations for MES, demonstrating the instability of the bound structure. Even when MES was bound in a similar fashion to OCS within the active site, the smaller alkane chain resulted in a shift of FMNH2 so that it was no longer in a position to catalyze the desulfonation of MES. The active site of SsuD requires a longer alkane chain to maintain the appropriate architecture for desulfonation.

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Current understanding of enzyme structure and function in bacterial two-component flavin-dependent desulfonases: Cleaving C–S bonds of organosulfur compounds

Liew,

Wicht,

Gonzalez

et al. 2024

Archives of Biochemistry and Biophysics

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Not as easy as π: An insertional residue does not explain the π‐helix gain‐of‐function in two‐component FMN reductases

Cited by 6 publications

References 33 publications

Oligomeric Changes Regulate Flavin Transfer in Two-Component FMN Reductases Involved in Sulfur Metabolism

Oligomeric Changes Regulate Flavin Transfer in Two-Component FMN Reductases Involved in Sulfur Metabolism

Shorter Alkanesulfonate Carbon Chains Destabilize the Active Site Architecture of SsuD for Desulfonation

Current understanding of enzyme structure and function in bacterial two-component flavin-dependent desulfonases: Cleaving C–S bonds of organosulfur compounds

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