A minimal RNA substrate with dual fluorescent probes enables rapid kinetics and provides insight into bacterial RNase P active site interactions

Bacterial ribonuclease P (RNase P) is a tRNA processing endonuclease that occurs primarily as a ribonucleoprotein with a catalytic RNA subunit (P RNA). As one of the first ribozymes discovered, P RNA is a well-studied model system for understanding RNA catalysis and substrate recognition. Extensive structural and biochemical studies have revealed the structure of RNase P bound to precursor tRNA (ptRNA) and product tRNA. These studies also helped to define active site residues and propose the molecular interactions that are involved in substrate binding and catalysis. However, a detailed quantitative model of the reaction cycle that includes the structures of intermediates and the process of positioning active site metal ions for catalysis is lacking. To further this goal, we used a chemically modified minimal RNA duplex substrate (MD1) to establish a kinetic framework for measuring the functional effects of P RNA active site mutations. Substitution of U69, a critical nucleotide involved in active site Mg2+ binding, was found to reduce catalysis >500-fold as expected, but had no measurable effect on ptRNA binding kinetics. In contrast, the same U69 mutations had little effect on catalysis in Ca2+ compared to reactions containing native Mg2+ ions. CryoEM structures and SHAPE mapping suggested increased flexibility of U69 and adjacent nucleotides in Ca2+ compared to Mg2+. These results support a model in which slow catalysis in Ca2+ is due to inability to engage U69. These studies establish a set of experimental tools to analyze RNase P kinetics and mechanism and can be expanded to gain new insights into the assembly of the active RNase P–ptRNA complex.


Introduction
2][3][4][5][6] RNase P occurs throughout phylogeny primarily as a ribonucleoprotein, which in Bacteria is composed of a ca.][10] As one of the first ribozymes discovered, RNase P has served as a model system for exploring RNA catalysis and molecule recognition.1][12] However, a complete model of the reaction cycle is currently lacking, but needed to fully understand how alternative substrates are bound and processed, and to understand the precise role and positioning of divalent ions in catalysis.
][20][21] The 5 0 and 3 0 ends of ptRNA are splayed and interact with different sites within the C-domain.The 3 0 RCC sequence of ptRNA pairs with conserved residues (G292,G293,U294) in the P15/16 internal bulge of RNase P. [22][23][24][25][26] The nucleotides N À1 N À2 adjacent to the cleavage site connect the acceptor stem and active site via a continuous stacking interaction in which they stack upon each other and with A333 in P RNA. 163][34] Chemical protection and FRET experiments, and cryoEM structures are also consistent with conformational changes in the C-domain that are involved in RNase P function, 16,33,35,36 but the molecular details are poorly understood.Deeper investigation of the RNase P substrate binding reaction and participation of active site residues is needed to provide the information necessary to develop mechanistic models that relate structure, kinetics, and biological function.
Minimal helical substrates, or minihelix substrates, represent a widely used and valuable experimental tool for investigating RNase P kinetics and active site interactions in vitro. 37inihelices have been particularly useful in defining RNase P metal ion cleavage requirements, 24,34,38,39 specificity, [40][41][42][43][44] for systematic investigation of functional groups at the cleavage site G 1 -C 72 and N À1 positions, 21,[45][46][47][48] small molecule screening, 49 and RNase P engineering. 50,51Similarly, small bipartite model substrates formed from annealing short oligonucleotides are also efficient substrates for bacterial RNase P. 43,52,53 However, most prior studies using model substrates primarily investigated reactions with the RNA subunit alone at high monovalent and divalent ion concentrations, which makes quantitative comparison and relating results to the biological context more challenging.Advantageously, synthetic RNAs are readily modified with fluorescent labels, nucleotide analogs, and isotopic substitutions and applied to RNase P holoenzyme reactions to provide deeper mechanistic insights into the kinetics of substrate binding, conformational changes, and transition state stabilization.
Here, we describe a minimal duplex substrate (MD1) for bacterial RNase P that facilitates incorporation of fluorescent probes permitting its use for mechanistic studies of substrate binding and catalysis.We used this tool to quantify the effects of mutations at the key active site residues in P RNA and provide evidence that G332 and A333, previously implicated in sequence specific interactions, contribute little to binding kinetics for this substrate.Remarkably, we found that mutations at U69 in P4 that were previously shown to result in large defects on RNase P activity, had minimal impact on substrate binding kinetics.Surprisingly, the effects of U69 mutation on catalysis were suppressed in Ca 2+ compared to Mg 2+ , which correlates with greater flexibility of U69 in Ca 2+ based on cryoEM structural analysis and SHAPE probing.Importantly, the results suggest that slow catalysis in Ca 2+ is due to an inability to engage in productive binding interactions with U69 and not intrinsic differences in transition state stabilization relative to Mg 2+ .

Results
Single turnover reaction kinetics of MD1 processing by E. coli RNase P The acceptor and T-stems of ptRNA are contacted by RNase P while the remainder of tRNA is dispensable for binding.However, impaired coaxial stacking of the acceptor and T-stems, or omission of the T-loop of ptRNA reduces cleavage rates e.g. 37,44,54In vitro studies show that, in general, truncated

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RSC Chemical Biology substrates bind with lower affinity due to loss of important enzyme-substrate contacts, although there are intriguing differences in the ability of RNase P enzymes to accept minimal substrates that are not fully understood. 44The MD1 substrate consists of a 21 nucleotide RNA oligonucleotide (5 0 2Ap(-2)-MD1) that forms a 12 basepair continuous helix with a complementary 16 nucleotide RNA (3 0 MD1) (Table 1, Fig. 2).When annealed, these two oligos form the stacked acceptor and T-stems of a well characterized B. subtillis tRNA Asp substrate including nine nucleotides of genomically encoded 5 0 leader and 3 0 GCCA sequence. 55Two different modifications were used to incorporate fluorescent probes for analysis of MD1 binding and kinetics.The 5 0 Cy3Ap(-2)-MD1 RNA contains a 5 0 Cy3 modification at the end of the 5 0 leader and allows MD1 and its 5 0 leader cleavage product to be visualized by denaturing PAGE, and binding kinetics to be measured using fluorescence anisotropy.2-Aminopurine (Ap) is an intrinsically fluorescent nucleobase that is quenched by base stacking. 56hus, since N À2 forms a stacking interaction with A333 in the E. coli RNase P active site, 16 we reasoned that a 2Ap modification at this position should be sensitive to such active site conformational changes.Accordingly, 2Ap was included at N À2

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to monitor changes in the environment of this nucleotide position.First, we determined the single turnover reaction kinetics and specificity for MD1 cleavage by E. coli RNase P under reaction conditions of 0.1 M NaCl, 17.5 mM Mg 2+ , and MES pH 6.These monovalent and divalent ion concentrations are optimal for the multiple turnover reaction (k cat /K m ) of native E. coli RNase P with an E. coli ptRNA Met substrate. 57Nonoptimal conditions of low pH were used to slow the catalysis so that the cleavage step could be measured by manual pipetting. 58The kinetics of formation of the 5 0 leader product were analyzed by denaturing PAGE and phosphorimager analysis.The 5 0 cleavage product co-migrated with a synthetic 5 0 -Cy3 labeled RNA oligonucleotide of the same sequence (MD.L), which is consistent with hydrolysis at the correct phosphodiester bond between U(-1) and G(1) (Fig. 2B).The kinetic data fit well to a single exponential function (eqn (1), Methods) over a range of 50-1500 nM RNase P (Fig. 2C).
The observed pseudo-first-order rate constant (k obs ) increased with RNase P concentration until a plateau is reached at 500 nM (Fig. 2D).The data are consistent with single substrate enzyme mechanism involving a second-order reaction (substrate binding) followed by irreversible product formation (Scheme 1).
The dependence of k obs on RNase P concentration was fit to this mechanism (eqn (2), Methods) in order to estimate the magnitude of k c and K 0 (where K 0 = k À1 /k 1 ) (Fig. 2E).The rate constant k c for conversion of ES to form EP was observed to be ca.0.017 s À1 , which is consistent with the value of 0.02 s À1 previously reported by Kirsebom and colleagues for a similar pATSerUG minihelix substrate, 59 and 0.0143 s À1 measured for a 3 bp minihelix substrate under similar conditions. 48These values for k c are also consistent with the value of 0.028 s À1 measured for native RNase P processing of an optimal ptRNA Met substrate. 60A K 0 of 189 nM was obtained by fitting the data in Fig. 2D to eqn (2) (Methods).This value is similar to the K d , app for binding of pATSerUG stem-loop substrate of 92 nM and a smaller substrate pMini3bpUG that has a K d , app of 150 nM, both measured in 40 mM Ca 2+ . 34Thus, MD1 is efficiently processed by E. coli RNase P with monophasic single turnover kinetics with reaction rate and apparent affinity matching comparable minimal substrates measured under similar reactions conditions.

Analysis of MD1 binding and cleavage using stopped flow fluorescence
Next, we used stopped-flow fluorescence to investigate the kinetics of binding and catalysis, and to measure the individual rate constants for association and dissociation in Scheme 1.The recent cryoEM structure of the E. coli RNase P complex with ptRNA showed that the first two nucleotides in the 5 0 leader sequence, N À2 N À1 , are bound in a pocket between conserved active site nucleotides A248 and A333. 16We reasoned that positioning 2Ap near the substrate cleavage site would be sensitive to binding and cleavage by RNase P. Mutagenesis experiments showed that A is the optimal nucleobase N À2 and G had only a small effect on k cat /K m . 16,61These results suggest that 2Ap at N À2 in the context of the 5 0 Ap(-2)-MD1 substrate will fit similarly into the same site in RNase P and report on association and cleavage kinetics.
To test the effect of RNase P binding on 5 0 Ap(-2)-MD1 fluorescence, we first measured the steady-state emission spectra of 100 nM substrate in the absence and presence of 1 mM RNase P (Fig. 3A).Ca 2+ was used as the divalent ion, which slows catalysis by ca.500-fold, allowing the emission spectrum of the ES complex to be acquired. 62The emission spectrum of 5 0 Ap(-2)-MD1 (l ex = 310 nm) is characteristic of 2-aminopurine with a broad peak with a maximum at ca. 365 nm. 56,63We observed that fluorescence intensity decreased upon addition of RNase P to a final concentration of 1 mM in the presence of 17.5 mM Ca 2+ , while the signal increased to even higher levels than for MD1 alone after 1 h of incubation at 17.5 mM Mg 2+ to completely convert substrate to product.These results are consistent with quenching of the 2Ap at N À2 in the ES complex and recovery of the signal upon substrate cleavage to form EP or rapid dissociation of the 5 0 leader.
To measure the kinetics of the 5 0 Ap(-2)-MD1 fluorescence during the reaction we used stopped-flow spectroscopy (Fig. 3B).RNase P and MD1 solutions were mixed to achieve final concentrations of 500 nM and 100 nM, respectively.Under these conditions, a rapid decrease in fluorescence was observed initially, followed by a slower increase in the fluorescence signal.We reasoned that the initial rapid decrease in signal likely reflects binding to form ES, which is consistent with the steady-state fluorescence results.The slower increase in fluorescence occured over a time scale similar to product formation observed by PAGE.To estimate the rate constants for the first and second phases (k obs1 and k obs2 , respectively) these data were fit to a double exponential function (eqn (3)).Values of 0.16 s À1 for k obs1 and 0.024 s À1 for k obs2 were measured for the data in Fig. 3B.To test whether the two fluorescence transients represent binding and catalysis, we used Ca 2+ as the divalent ion which slows catalysis with minimal effect on binding steps. 62When Ca 2+ was used as the divalent ion, a fast decrease in 2Ap fluorescence was still observed (Fig. 3C and D).However, the subsequent increase in signal observed with Mg 2+ was absent for up to 200 seconds.Under these conditions, there was minimal product formation detectable by PAGE (see below).Thus, the rapid decrease in fluorescence in Fig. 3B is likely to reflect binding or a conformational change after binding, while the slower increase in fluorescence is attributable to substrate cleavage.
To validate this model and estimate rate constants for individual reaction steps we acquired time-dependent fluorescence data using E. coli RNase P concentrations of 500 nM, 750 nM, and 1000 nM (Fig. 4A).The magnitudes of k 1 and k À1 could be evaluated only under a limited range of RNase P Scheme 1

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RSC Chemical Biology concentrations since the decrease and subsequent increase in signal due to binding and catalysis largely offset each other below 500 nM.At RNase P concentrations greater than 1000 nM binding becomes difficult to measure accurately due to instrument dead time limitations (i.e. the interval between mixing and the start of data collection).Nonetheless, these data were sufficient to estimate reaction rate constants by global fitting to the kinetic model shown in Scheme 1, assuming scaling factors to account for the expected signal differences for S, ES, and EP (Fig. 4A).A plot of k 1 , k À1 , and k 2 values obtained from global fitting versus RNase P concentration shows that k 2 and k À1 were essentially independent of RNase P concentration consistent with unimolecular reactions.In contrast, the magnitude of k 1 increased with increasing enzyme concentration, which is characteristic of bimolecular association (Fig. 4C).The data are consistent with a second-order rate constant for substrate association, k 1 , of 0.43 Â 10 6 M À1 s À1 .The fitted value for the cleavage step, k 2 , of 0.019 s À1 matches the value of 0.017 s À1 measured by single turnover kinetics using PAGE (Table 2).The value of k À1 of 0.084 s À1 is consistent with a near rapid equilibrium single turnover mechanism in which the K 0 of 184 nM observed by fitting the enzyme concentration dependence of k obs (Fig. 2E) is equivalent to Assuming this mechanism, we note that the observed rate constant for association k 1 of 0.43 Â 10 6 M À1 s À1 and dissociation rate constant k À1 of 0.084 s À1 from global fitting predicts a K 0 of 195 nM that is within error of 189 nM measured by single turnover kinetics using PAGE.Since analysis of 5 0 Ap(-2)-MD1 kinetics using 2Ap fluorescence was limited to a narrow concentration range we took advantage of the 5 0 -Cy3 modification of 5 0 Cy3Ap(-2)-MD1 to further test whether the initial fluorescent transient detected by 2Ap fluorescence accurately measures substrate association kinetics.We reasoned that due to the small molecular weight of MD1 as compared to the much larger RNase P, association kinetics for MD1 should be detectable by fluorescence anisotropy.Therefore, we collected the steady-state emission spectra of 5 0 Cy3Ap(-2)-MD1 free in solution, bound to RNase P in the

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presence of Ca 2+ , and under rapid cleavage conditions in Mg 2+ .
In contrast to the significant changes in the 2Ap signal, the Cy3 fluorescence intensity was minimally sensitive to binding and cleavage by RNase P (Fig. 5A).However, when 5 0 Cy3Ap(-2)-MD1 was combined with RNase P to achieve final concentrations of 100 nM substrate and 1000 nM enzyme, a rapid increase in anisotropy was observed that is consistent with the association of MD1 with the significantly larger ribonucleoprotein enzyme.
The increase in anisotropy occurred with an observed pseudofirst-order rate constant of ca.0.23 s À1 , similar to the observed k 1 obtained with the 5 0 Ap(-2)-MD1 substrate at the same concentration (1000 nM) (Fig. 5B).
The rate constants for association and dissociation estimated by global fitting of stopped-flow fluorescence data using 5 0 Cy3Ap(-2)-MD1 reflect a small commitment to catalysis (C f = k 2 /k À1 = 0.017 s À1 /0.084 s À1 = 0.2). 64Thus, the K 0 value determined from fitting single turnover data approximates the dissociation constant for binding (K d ).Using this framework, we next investigated the effects of a series of active site mutations to quantify their contributions to binding and catalysis, which will help to guide a detailed inhibitor characterization and structure-function studies at a chemical level.

Multiple turnover reaction kinetics of MD1 processing by E. coli RNase P
Steady state kinetics are important for understanding biological specificity, competition between alternative substrates, and for screening assays.Therefore, to determine the Michaelis-Menten kinetic parameters k cat , K m and k cat /K m for MD1 cleavage, we positioned a BHQ2 modification at the 3 0 end of 5 0 Cy3Ap(-2)-MD1 to quench the fluorescence of Cy3 in the substrate and undergo an increase in fluorescence upon formation of the cleaved product.Accordingly, we collected the steady-state emission spectra of 5 0 Cy3Ap(-2)BHQ-MD1 free in solution under reaction conditions, bound to RNase P in the presence of Ca 2+ to slow catalysis, and under cleavage conditions in Mg 2+ (Fig. 6A).While there is a small change in fluorescence intensity upon formation of ES, a much larger increase in fluorescent signal occurs concomitant with formation of EP.
Using this information, we confirmed that the increase in Cy3 signal upon product formation observed with 5 0 Cy3Ap-(-2)BHQ-MD1 is consistent with the kinetics of this step observed by monitoring the 2Ap modification at N À2 .Stopped flow fluorescence experiments measuring Cy3 emission upon mixing 5 0 Cy3Ap(-2)BHQ-MD1 and RNase P to achieve final

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concentrations of 100 nM and 1000 nM, respectively, showed the expected large increase in fluorescent signal that is associated with product formation.The increase in signal occurred with an observed rate constant of 0.026 AE 0.05 s À1 (Fig. 6B), consistent with the k 2 of 0.019 s À1 from global fitting of 5 0 Ap(-2)-MD1 fluorescence (Fig. 4).In order to determine the multiple turnover kinetics of MD1 we took advantage of the large signalon change in Cy3 fluorescence of 5 0 Cy3Ap(-2)BHQ-MD1 upon cleavage by adapting it to a plate reader assay.As described in Methods, individual wells contained aliquots of substrate at different concentrations that were mixed with enzyme using an integrated injector.Individual time courses of the increase in fluorescence due to product formation were recorded for reactions containing constant (50 nM) 5 0 Cy3Ap(-2)BHQ-MD1 and increasing concentrations of 5 0 Ap(-2)-MD1.The primary data for a reaction containing 1 mM substrate is shown in Fig. 6C.
The initial rates determined from individual time courses were fit to the Michaelis-Menten equation to estimate k cat and K m (Fig. 6D).The value of 0.5 AE 0.1 s À1 for k cat at pH 8 is 20-25 fold faster than the value of k c of 0.017-0.022s À1 measured at pH 6.0.This difference is consistent with the pH dependence of RNase P cleavage which follows general base catalysis with a kinetic pK a at pH 6.5-8. 32,65The value of 1.8 AE 0.4 mM for K m is also significantly higher than the magnitude of the analogous quantity K 0 determined using single turnover kinetics.
Importantly, the K 0 measured at pH 6 was shown to approximate Therefore, the large magnitude of k cat contributes to the comparatively large K m compared to K 0 , which more closely reflects equilibrium binding affinity.

Differential effects of mutations at active site nucleotides on binding and catalysis
Using MD1 as a substrate we measured the effects of mutations in E. coli P RNA at nucleotides contacting the ptRNA cleavage site in the ES complex or involved in catalytic metal ion binding.As illustrated in Fig. 1 the 3 0 RCCA sequence common to tRNA binds to the P15/16 internal loop between P15 and P16, and distal nucleotides in the 5 0 leader are contacted by rnpA protein.With respect to nucleotides directly flanking the cleavage site, three separate regions of P RNA combine to form the active site.These include A248 in J5/15, G332 and A333 in J18/2, and a divalent metal binding site in P4 involving G68 and U69 (Fig. 7A).The interactions between A248 and N À1 are understood in some detail. 20,21,66A recent cryoEM structure of E. coli RNase P bound to ptRNA shows an optimal U À1 , which is the optimal base at this position, contacts the Hoogstein edge of A248 with a distance of 2.8 Å between the U À1 O4 and N6 of A248. 16The roles of G332 and A333 are less well understood, but likely contribute to binding, recognition, and/or Paper RSC Chemical Biology positioning of the ptRNA leader.The E. coli RNase P-ptRNA complex structure reveals that the N À1 and N À2 bases stack together in a pocket formed by A248, A333, and P4.The leader nucleotides N À3 and N À4 , are in position to contact the Hoogstein edges of G332 and A333, although the precise interactions are not resolved. 16The cryoEM density of the ES complex indicates flexibility distal to N À2 of ptRNA, and the structural details and functional importance of interactions further out in the 5 0 leader remain unclear.Therefore, we used the MD1 substrate to compare the effects of mutation at A248, G332, and A333 on binding affinity, kinetics, and catalysis.Previous studies of E. coli RNase P demonstrated that A248G and A248C mutations had relatively minimal effects on binding and catalysis in reactions using high monovalent ion concentration where the P RNA alone is catalytic. 20,66In contrast, a A248U mutation exhibited only a 2-6-fold effect on catalysis in previous studies, but ranges from a 300-fold impact on binding at 25 mM Mg 2+ to a smaller effect at higher concentrations (800 mM Mg 2+ ). 20,66Similarly, mutations in J18/2 have also been analyzed for P RNA alone reactions at high ionic strength conditions, 67 but their contribution to RNase P holoenzyme reactions is poorly understood.The positions homologous to G332 and A333 are conserved among P RNAs as purines (Fig. 7B) although U occurs at G332 in P RNA from Thermotoga species.The nucleotide sequence AGA in J18/2 is universally conserved as is the sequence AU which flanks A333 and G332 on either side.These residues are involved in tertiary contacts within the folded P RNA structure and are distal to the bound substrate relative to A333 and G332.Therefore, we initially examined the effects of A248U, G332U, and A333U mutations on 5 0 Cy3-MD1 cleavage by quantifying product formation using PAGE.
The results showed that an A248U mutation results in a dramatic decrease in MD1 product formation, consistent with previous studies (Fig. 7C). 20,66The slow reaction rate is in line with the expectation based on previous results of a 300-fold increase in K d that would result in a predicted value of ca.40 mM for MD1. 20However, recent studies of A248U under conditions optimal for catalysis by P RNA alone (0.8 M ammonium acetate, 100 mM Mg 2+ ) increase sensitivity to T1 cleavage in P18 consistent with an indirect effect on function due to local misfolding. 66Surprisingly, we observed that an A333U mutation has minor effects on K 0 and k c , consistent with the residue's structural importance but not indicative of fundamental substrate interactions nor an essential role for a purine at this position.Similarly, G332U single turnover kinetics are essentially indistinguishable from native E. coli RNase P.These results are consistent with a role for A248 in positioning the reactive phosphate in the active site.The results suggest only minor roles for specific functional groups of G332 and A333 in substrate binding and are more generally consistent with a role for A333 in stacking.

Mutations in P4 uncouple binding and catalysis
8][29][30][31] Despite important steps forward in pinpointing key functional groups in P4 and the C-domain involved in Mg 2+ binding, previous studies focused primarily on the contribution to the chemical step and not effects on binding.Moreover, most data are derived from the reactions of the P RNA subunit alone under high monovalent or divalent ion conditions or using engineered non-native constructs.
Therefore, to further resolve the contribution of U69 and P4 to binding kinetics and catalysis we investigated previously characterized P4 mutations (U69A and C70U) on MD1 cleavage by the E. coli RNase P holoenzyme using PAGE and stopped flow assays.Previous studies with P RNA alone under high salt conditions showed that a U69A mutation does not alter the pattern of base-pairing in P4 and results in only a fivefold reduction in k c . 30,68This result suggests the a key role of U69 in maintaining the bulged helical structure of P4.However, a 4-thiouridine modification of U51, the homologous residue in B. subtilis P RNA, had a much larger effect on catalysis 29 underscoring the need for further information on its role.A C70U mutation was identified by in vitro selection for E. coli P RNA with faster reactivity in Ca 2+ versus Mg 2+ from a pool of ribozymes randomized in P4. 69 However, these studies used a fused self-cleaving RNase P-tRNA construct in high monovalent ion conditions (2 M), and did not include quantitative studies on ptRNA processing or holoenzyme reactions.Thus, a more detailed investigation of these mutants can reveal important new features of RNase P active site divalent ion specificity.
To quantify the effects of U69A and C70U mutation on binding affinity and catalysis we used single turnover reactions to estimate k c and K 0 .We also used stopped-flow fluorescence for analysis of the kinetics of 5 0 Ap(-2)-MD1 to measure association and cleavage kinetics.PAGE analyses of reaction products was consistent with cleavage at the correct site although low substrate conversion precludes detection of minor cleavage products (Fig. 8A).In single turnover reactions the k obs was saturated at relatively low enzyme concentrations for both mutants consistent with minimal effects on substrate binding (Fig. 8B).The effects of both mutations on catalysis were significant under these conditions with U69A resulting in a ca.10-fold decrease in k c and C70U a ca.250-fold reduction.The data are consistent with a K 0 of less than 250 nM which would be in the range of the wild type enzyme.However, the very slow rate constants at low enzyme concentrations (o0.0001 s À1 ) were difficult to measure with precision limiting our ability to quantify K 0 for these mutants.Therefore, we analyzed the binding and cleavage of C70U and U69A mutant RNase P enzymes by stopped flow fluorescence using the same 5 0 Ap(-2)-MD1 substrate (Fig. 8C and D).Both U69A and C70U mutants showed the initial rapid decrease in fluorescence associated with substrate binding.These data fit a single exponential function with observed rate constants of 0.32 s À1 and 0.35 s À1 for U69A and C70U, respectively, that are comparable to the value of 0.16 s À1 for k obs1 for native RNase P measured under the same conditions (Fig. 3B).Thus, the large defects in the substrate cleavage step engendered by U69A and C70U RSC Chemical Biology Paper mutation are independent from the change in 2Ap fluorescence at N À2 that is induced by RNase P association.
Evidence that slow catalysis in Ca 2+ is due to altered active site structure The C70U mutation was isolated by Pace and colleagues from a SELEX experiment and a self-cleaving P RNA-ptRNA conjugate designed to select for P RNA mutants with faster cleavage rates in Ca 2+ . 69C70U mutation resulted in a similar k obs for reactions in Ca 2+ versus Mg 2+ , but also caused a decrease in activity independent of divalent ion type.These experiments were performed with a non-native construct, with the RNA alone, under high monovalent ion concentration (1 M).To better understand the functional effects of the C70U mutation on metal ion specificity we measured the k c for the C70U and U69A mutants in the context of the E. coli RNase P holoenzyme in Ca 2+ under saturating enzyme concentrations (Fig. 9A).Surprisingly, the effect of both mutations on the observed k c for MD1 reactions in Ca 2+ was relatively small compared to Mg 2+ .The lack of effect of U69 mutations on k c in Ca 2+ could be due to a change in the rate-limiting step, or a difference in the role of U69 in active site interactions involving Ca 2+ versus Mg 2+ .Previous biochemical data and cryoEM studies showed that the structure of E. coli RNase P holoenzyme is essentially identical in both Mg 2+ and Ca 2+ , although one or more changes in critical structural elements or cumulative small effects due to differences throughout the P RNA are possible.Among these differences we noted that U69 has weak cryoEM map features in both the free E. coli RNase P holoenzyme and the ES complex when Ca 2+ is used as the divalent ion (Fig. 9B).This observation suggests that the insensitivity of U69 to mutation in Ca 2+ could be due to its increased flexibility in Ca 2+ and failure to productively engage in divalent ion interactions.
To further investigate the flexibility of U69 and differences in P RNA structure in Mg 2+ and Ca 2+ we performed SHAPE mapping of E. coli P RNA (Fig. 9C). 70,71The overall pattern of modification in both divalent ions occurred in loops, bulges, and single-stranded regions that are consistent with the folded structure of P RNA.There were 46 modifications sites that were common in both Mg 2+ and Ca 2+ while 38 additional modifications were detected in Ca 2+ compared to 15 nucleotides where SHAPE reactivity was greater in Mg 2+ .Both common and Mg 2+ -

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or Ca 2+ -specific modifications sites were detected throughout E. coli P RNA.In some regions the results are consistent with overall higher reactivity in Ca 2+ with additional modifications detected at nucleotides adjacent to positions where SHAPE reactivity occurs in both ions (e.g.47-50 in P3; 93-98 in L8; 214-215 in L14; and 314-316 in L18).However, there were three regions (J5/15, P15-P16, and P4) in the C-domain of P RNA where the pattern of reactivity changed within structures that form the active site.
The most extensive difference in modification pattern occurred in the P15-16 internal bulge that binds the 3 0 RCC sequence of ptRNA where reactivity observed in Mg 2+ was suppressed by Ca 2+ (292-294) except of A295 which showed an increase in modification in the presence of Ca 2+ .P15-16 has been shown to bind divalent ions and contribute to interactions that are important for RNase P catalysis.Based on available structures of bacterial RNase P bound to ptRNA and tRNA, however, it does not appear as though P15-P16 directly contacts ions that also interact with the reactive phosphoryl group.
A shift in the reactivity in J5/15 is observed as well from A248 in Mg 2+ to A249 in Ca 2+ .Also, in the presence of Ca 2+ , there is increased reactivity in P4 at G68 and A66 and suppression of reactivity observed with Mg 2+ at A11 in the P1-P4 helical junction proximal to U69.Thus, both cryoEM data and SHAPE mapping are consistent with greater flexibility of U69 in the presence of Ca 2+ .This greater flexibility correlates with the 300fold slower k c observed in Ca 2+ relative to Mg 2+ which is likely due, at least partially, to a reduced ability of Ca 2+ to engage U69 in binding interactions.This result suggests a rationale for the minimal effects of U69A and C70U mutations on k c in Ca 2+ versus Mg 2+ in which the effects of mutation seen at U69 in the presence of Mg 2+ is suppressed in the presence of Ca 2+ because the latter cannot cooperate with U69 in promoting catalysis.

Discussion
Here we report the detailed reaction kinetics of a minimal duplex substrate for bacterial RNase P with dual internal and

RSC Chemical Biology Paper
terminal fluorescent probes and illustrate its use for gel-based assays as well as equilibrium and stopped flow fluorescence spectroscopy.As illustrated previously for similar minimal substrates for bacterial RNase P, 49 MD1 is further adaptable to fluorescence based plate reader assays for high throughput screening and follow on mechanism of action studies.As an initial application we employed MD1 to quantify the effects of mutations at the key P RNA active site residues, and revealed that, contrary to previous models, G332 and A333 are unlikely to participate in sequence-specific interactions with the MD1 5 0 leader. 10We further demonstrated that mutations at U69 in P4, a key active site metal ion contact, uncouples substrate binding and catalysis.Surprisingly, the effects of U69 mutation on catalysis were minimized when Ca 2+ replaced Mg 2+ in the reaction, which correlates with greater flexibility of U69 in Ca 2+ observed by cryoEM density analysis and SHAPE.Taken together, these new data suggest that stabilizing interactions involving U69, that occur with Mg 2+ that are susceptible to mutation, are missing in Ca 2+ .This result runs counter to previous mechanistic interpretation of slower RNase P catalysis in Ca 2+ relative to Mg 2+ in terms of chemical differences in nucleophilic activation. 62,72The results further demonstrate a facile analytical tool for dissecting active site interactions and the involvement of key enzyme and substrate functional groups using chemical and isotopic substitutions for mechanistic studies.
Minimal versions of tRNA have been widely used to investigate the structure and function of tRNA modifying enzymes and tRNA binding proteins.In 1989 Franklyn and Shimmel showed that a ''minihelix'' derivative of tRNA composed of the stacked amino-acid acceptor-TCC stems was a substrate for alanine tRNA synthetase. 73Other minimal minihelix substrates consisting of the acceptor and anticodon stems as well as miniduplexes like MD1 have also been developed as tools for analysis of aminoacyl tRNA synthetases structure and function e.g., 74,75 as well as EF-Tu. 76,77They have continued to serve as useful tools for these and other enzymes and tRNA binding proteins. 78,79imilar minihelix or miniduplex substrates have been successfully used to investigate bacterial RNase P and provided significant insights into interactions at the cleavage site, roles and interactions of divalent ions, and principles for engineering P RNA for therapeutic applications.Using SELEX to discover novel substrates Pan and colleagues used a circular RNA pool to discover short stem loop and duplex substrates for P RNA ribozyme reactions, thus demonstrating inherent specificity for such alternative substrates. 80Small bipartite model substrates were shown to be substrates for E. coli and T. thermophilus RNase P enzymes, however, there are significant defects in processing due to sequence length and structure. 44ven smaller 3bp stems have been used to probe the contribution of TPsiC stem loop interactions. 34,48Acceptor stem duplexes containing only a three-nucleotide 5 0 leader are efficient minimal substrates for E. coli and B. subtilis RNase Ps enabling biophysical studies of nucleotide conformations and metal ion interactions at the cleavage site. 53,81With respect to probing active site interactions a model hairpin-loop substrate pATSer has been extensively used by the Kirsebom laboratory, initially to investigate the roles of metal ions in catalysis and identify nucleotides and functional groups involved in 5 0 and 3 0 end recognition. 11,13These studies took full advantage of the ability to site-specifically embed functional group modifications at the atomic level to probe the interactions at the substrate cleavage site. 38,39,45,48,59,82Using pATSer these researchers showed the importance of N À1 the N 1 -N 73 base pair and importance of the T-loop sequence for PRORP. 83uplex and minimal substrates have also been adopted to engineer RNase P specificity and for drug discovery.E. coli P RNA fused to additional 3 0 guide sequences results in the potential to form an intermolecular duplex substrate that can be used to target RNAs for cleavage through hybridization with target sequences. 51,84These guide RNA containing P RNAs (M1GS) have been shown to provide useful tools to hydrolyze human and viral mRNAs in order to decrease gene expression and virus replication. 85For discovery of small molecule inhibitors Torres-Larios and colleagues used a small minihelix substrate incorporating an Alexa fluorophore and quencher on the 3 0 and 5 0 ends, respectively, for which cleavage results in a signal-on assay for high-throughput screening.A key advantage of such minimal substrates is avoidance of potential false positives due to small molecules that inhibit the reaction by binding to structural elements of tRNA instead of binding to the target enzyme RNase P, although the loss of interactions important for ptRNA binding when using minimal substrates could engender some risk of false negatives (e.g.loss of small molecules that bind to the S domain of RNase P RNA to inhibit interaction with the tRNA T loop). 49Thus, the information gained from detailed kinetics of minimal and alternative substrates can be useful in engineering the P RNA ribozyme activity for therapeutic applications and deeper understanding of effects of inhibitors on reaction kinetics.Our studies using MD1 build directly on the success of these studies by incorporating terminal and internal fluorescent probes allowing multiple modes of detection.This capability permits direct comparison of results across a range of methods including traditional kinetics assays using PAGE, rapid kinetics, and high throughput assays.
The analysis of a set of previously characterized active site mutants using the MD1 substrate are consistent with the wellestablished roles of A248 and U69 in bacterial RNase P enzyme function.Biochemical and structural data indicate direct interaction between nucleotides G332 and A333 in J18/2 and nucleotides proximal to the cleavage site. 10,16,35,86,87Yet, mutating these conserved purines to U did not provide evidence for significant contributions to 5 0 leader recognition or catalysis.Based on miscleavage results observed using substrates containing a 2 0 -deoxy modification at N À1 we proposed that A248 forms a cis WC/WC base pair with N À1 . 20However, studies aimed at testing N À1 and A248 interactions using extensive chemical modification of minimal substrates showed that sensitivity to modification was substrate dependent, but largely inconsistent with a cis WC/WC interaction. 66The cryoEM

Paper
RSC Chemical Biology structure of E. coli RNase P bound to two alternative substrates with different nucleotides at N À2 /N À1 revealed that for both dinucleotides the WC edge of N À1 in fact contacts the Hoogsteen edge of A248 while N À2 is sandwiched between N À1 and A333 such that a continuous three nucleotide helical stacking geometry forms in the order 5 0 -A333/N À2 /N À1 -3 0 .Thus, mutation of either G332 or A333 to U should not interfere with a role in stacking interactions that position the substrate in the active site.However, the results with MD1 alone do not rule out sequence specific interactions between G332 and A333 for some alternative substrates.The central role of P4 and the universally conserved bulged U in binding catalytic metal ions is well established.However, key questions remain regarding the number and roles of divalent ions involved directly in transition state stabilization.The model for RNase P catalysis is based on a chemically feasible two metal ion model and kinetic assays as well as biophysical studies support the participation of two or more divalent ions in transition state stabilization.However, most previous studies of P4 metal ion interactions were performed using the P RNA ribozyme alone, typically at high monovalent and divalent ion concentrations.Although foundational these conditions could obscure or enhance interactions important in holoenzyme reactions.Also, since these studies focused on the role in catalysis, they used single turnover reaction conditions to minimize the contributions of substrate binding.Taking advantage of the ability to measure rapid kinetics we demonstrate that mutations at U69 in P4 resulting in large defects in catalysis nonetheless have minimal impact on the rate constant for substrate binding.This result suggests that Mg 2+ interactions involving U69 in the transition state may not necessarily be populated in the ground state pre-catalytic complex (ES*).The current mechanistic model for RNase P binding involves a conformational change that forms the coordination site for an essential but weakly binding catalytic metal ion.The results here are consistent with even weaker binding of this ion or class of ions due to U69 mutation resulting in accumulation of ES* with minimal effects on the steps for its formation.
Interestingly, the effects of mutation, previously indicated to affect the ability of U69 to participate in catalytic metal ions interactions, diminish in Ca 2+ .As an alternative divalent ion Ca 2+ has been used widely in the investigation of RNase P to slow the cleavage step without large effects on the structure of the ES* complex.This interpretation is supported by biochemical studies 62,[88][89][90][91][92] and comparison of the crystal structure of T. maritima RNase P solved in Mg 2+ and cryoEM structure of E. coli RNase P ES* complex assembled in Ca 2+ . 15,16However, the mechanistic basis for slower cleavage in Ca 2+ has not been established.Early studies which demonstrated the use of substituting Ca 2+ to slow cleavage and distinguish binding and catalysis suggest a connection with divalent ion pK a .The higher pK a for deprotonation of a water molecule in the hydration sphere of Ca 2+ compared to Mg 2+ (12.7 versus 11.4) provided a rationale for slower catalysis as the direct result of lower concentration of metal-hydroxide which acts as a nucleophile or general base to accept a proton from water.
However, the results presented here together with previous cryoEM and mutagenesis data provide an alternative explanation for slower catalysis in Ca 2+ and why this effect is uncoupled from binding.CryoEM data and SHAPE analysis of E. coli P RNA are consistent with greater flexibility of U69 in the free holoenzyme and that persists in the ES* complex.This greater flexibility suggests that Ca 2+ fails to engage in productive interactions with U69 as the cause of slower cleavage.As demonstrated by stopped flow analysis, both U69A and C70 showed native substrate binding kinetics in Mg 2+ despite large effects on catalysis.Since the metal ion interactions involving U69 contribute primarily in the transition state, the inability of Ca 2+ to engage U69 productively does not affect binding.Similarly, mutations altering U69 function in Mg 2+ have little effect on catalysis in Ca 2+ because it makes a different or restricted set of interactions in which U69 participates less.That is, the stabilizing interactions involving U69 that occur with Mg 2+ that are susceptible to mutation are missing in Ca 2+ .

Methods
Preparation of RNAs and holoenzyme assembly RNA oligonucleotides (Table 1) were obtained commercially (Horizon Dharmacon) and deprotected according to vendor protocol.The 3 0 MD1 RNA oligo was used for all MD1 substrates which differed according to the desired 5 0 fluorescent probe modification (5 0 Ap(-2)-MD1; 5 0 Cy3-MD1, 5 0 Cy3Ap(-2)-MD1, or 5 0 Cy3Ap(-2)BHQ-MD1).To prepare duplex MD1 substrates the 3 0 MD1 RNA was combined with the appropriate complementary RNA at a ratio of 1 : 1-1 : 2 in reaction buffer (MES pH 6 or Tris pH 8; 100 mM NaCl, 0.15% Triton x-100) and incubated at 95 1C for 3 minutes then transferred to 37 1C for 10 minutes.An aliquot of concentrated MgCl 2 or CaCl 2 solution was added to achieve the desired concentration, and the incubation continued for an additional 10 min at 37 1C.The E. coli RNase P RNA subunit was synthesized by in vitro transcription using T7 polymerase from a plasmid DNA template, and purified by one of two methods-denaturing PAGE or native size exclusion chromatography (SEC).The denaturing urea-PAGE method used 6% polyacrylamide gels in TBE buffer, visualization by UV shadowing, and passive elution of the excised RNA band into 40 mM Tris pH 7.5, 10 mM EDTA, 1% SDS.Eluted RNA was recovered by ethanol precipitation after phenol/chloroform extraction. 93For the SEC method, P RNA was purified after in vitro transcription using an AKTA PURE instrument and Hiload 16/600 Superdex 200 pg column with isocratic elution TE buffer (10 mM Tris pH 7.5, 1 mM EDTA).The eluted RNA was stored at À20 1C.
The E. coli C5 protein was affinity purified using the NEB IMPACT system.The C5 protein was overexpressed as a chitinbinding domain fusion with subsequent removal of the tag by intein cleavage followed by dialysis and concentration as previously described. 57 Equilibrium and stopped-flow fluorescence spectroscopy Steady-state spectra of MD1 assembled using the 5 0 Cy3Ap(-2)-MD1 RNA oligo were measured for the following samples.Substrate: Prepared as described above at a concentration of 100 nM of MD1.ES Complex: 100 nM MD1and 1 mM RNase P in reaction buffer containing 17.5 mM CaCl 2 .Enzyme plus Product: 100 nM MD1and 1 mM RNase P in reaction buffer containing 17.5 mM MgCl 2 .The Enzyme plus Product sample was incubated at 37 1C for 1 hour to achieve complete conversion of ptRNA.Samples were maintained at 37 1C for the duration of the experiment.Spectra were acquired using a thermostatted Carey Eclipse fluorescence spectrometer.Scans were taken in a 5 mm Â 5 mm cuvette at 37 1C from 320-450 nm with an excitation wavelength of 305 nm, emission slits at 5 nm, and a scan rate of 120 nm min À1 .Three spectra were averaged, and an averaged spectrum of a background control was subtracted to yield the final spectra.The time dependence of changes in the fluorescence of 2Ap and Cy3 labels in MD1 were measured by stopped-flow fluorescence spectroscopy using an Applied Photophysics SX20 instrument equipped with LED light sources (300 nm for 2Ap, and 535 nm for Cy3) in a single mixing (two syringe) mode.Power supply outputs were varied between 2 and 12 mA depending on the duration of the kinetics to optimize sensitivity and minimize photobleaching.Photobleaching was evaluated by comparing rate constants obtained at different LED outputs.Emission was measured using a high pass filter (320 nm for 2Ap and 570 nM for Cy3).Temperature was maintained at 37 1C using a circulating water bath connected to the sample handling unit.Equal volumes of RNase P and MD1 solutions, each at 2Â the respective final concentration, were mixed to yield a total drive volume of 140 mL.Stopped flow kinetic were initially analyzed using a double exponential function to estimate the rate constants for the first and second reaction phases.
Global data fitting and analysis were performed using KinTek Explorer v11 (KinTek). 94Fluorescence anisotropy measurements were performed with the instrument's T-format excitation and emission polarizer accessory.Samples were excited using the 535 nm LED and the vertical and horizontal polarized light emission was monitored at 901 using 570 nm long-pass filters on both detectors.To correct for gain differences in the two detection channels a G-factor was determined prior to running the experiments using the SX software.The observed rate constant reflecting binding was determined using the single exponential function (eqn (1)) in Origin 8.5.

Fluorescence microplate reader assay of multiple turnover kinetics
The fluorescence signal of the 5 0 Cy3Ap(-2)BHQ-MD1 RNA substrate is quenched due to the presence of a 3 0 modification with BHQ2.To measure this signal for multiple turnover kinetics we used a BMG Clariostar microplate reader and mixed separate solutions at twice the intended final concentration using the instrument's injector.Final substrate concentrations were 50 nM-5 mM 5 0 Cy3Ap(-2)BHQ-MD1 and 10 nM E. coli RNase P. First, 30 mL of 2x substrate in Tris pH 8; 100 mM NaCl, 0.15% Triton x-100 was pipetted into the wells of a 90 well black low-bind microplate (Corning 3684).A range of concentrations were used to survey substrate limiting and saturating conditions (50 nm-5 mM).To start the reactions 30 mL of 2x enzyme solution in the same buffer was injected into each well that contained substrate.After 5 seconds of shaking to mix the solutions, the Cy3 fluorescence intensity was measured for each well with a cycle time of 30s.The initial and final fluorescence intensities were determined by fitting the data to eqn (1).Using these values the amplitude was normalized and the first 10% of the data was fit to a linear function and the slope determined by fitting was used to calculate v obs in units of nM s À1 for each substrate concentration.

Paper RSC Chemical Biology
In vitro SHAPE analysis DNA oligonucleotides for primer extension were 5 0 end labeled with g-32 P-ATP and polynucleotide kinase followed by gel purification by denaturing urea-PAGE on 20% polyacrylamide gels.SHAPE reactions contained 100 nM RNase P and 500 nM ptRNA was added to probe the structure of the ES complex.Binding reactions in standard reaction buffer containing Ca 2+ or Mg 2+ as indicated in the text were conducted.5 mL of Nmethylisatoic anhydride (NMIA) stock was added to 45 mL RNase P in Mg 2+ , or Ca 2+ , of the RNase P-ptRNA complex in Ca 2+ .The modified RNA was recovered by ethanol precipitation, and resuspended in 10 mL 10 mM Tris pH 7.5 and 1 mM EDTA for subsequent primer extension mapping. 70The samples were resolved using 8-10% denaturing PAGE gels, then scanned by phosphorimager and individual band intensities were quantified using the SAFA (Semi-Automated Footprinting Analysis) program. 95The absolute NMIA reactivity for each sample was measured at each position by subtracting the no NMIA control intensities band intensities of the NMIA reacted samples intensities.The control and NMIA reacted intensities were normalized assuming low intensity reflects unreactive positions, and common thresholds for high and low reactivity for the two data sets were established as described. 71

Fig. 1
Fig. 1 Ribonuclease P structure and interactions with substrate ptRNA.(A) Ribonuclease P (RNase P) catalyzes the maturation of tRNA precursors (ptRNAs) via a site-specific endonuclease cleavage to generate the mature tRNA and free 5 0 leader product.(C) CryoEM structure of E. coli RNase P bound to pre-tRNA Met ; colored according to panel B. The P RNA subunit consists of the specificity domain (S-domain, orange) and the catalytic domain (C-domain, blue) which includes the P15/16 internal bulge that binds the ptRNA 3 0 RCCA sequence.(D) Detail of the E. coli RNase P holoenzyme active site.The ptRNA, P RNA and C5 are colored the same as in panel C and the reactive phosphoryl group is shown as a yellow sphere.The complementary strand of the acceptor stem including the 3 0 ACCA sequence is not shown for clarity.

3 0 MD1 5 0 5 0 5 0 5 0 5 0 9 Fig. 2
Fig. 2 Sequence and single turnover kinetics of MD1 cleavage by E. coli RNase P. (A) Design and sequence of MD1 substrate consisting of two annealed synthetic RNA oligonucleotides.The nucleotides in ptRNA consisting of the stacked acceptor and TCC stem included in MD1 are boxed, and a red arrow indicates the RNase P cleavage site.(B) PAGE analysis of products from a reaction containing 50 nM 5 0 Cy3-MD1 and 1 mM E. coli RNase P. The positions in the gel of the annealed MD1 duplex and the 5 0 fragment generated by RNase P cleavage are shown on the left.Lane M contains equal amounts of the annealed MD1 substrate and a synthetic RNA oligo matching the expected cleavage product (Table 1).(C) Plot of fraction (F) of product formed from total substrate concentration ([P]/([P] + [S])) determined by phosphorimager analysis versus time.These data are fit to an exponential function (eqn (1), Methods) to determine k obs .(D) Dependence of k obs for MD1 single turnover reactions as a function of increasing E. coli RNase P concentration.These data are fit to an equation for Scheme 1 involving equilibrium binding followed by the substrate cleavage step (eqn (2), Methods; k c = 0.017 s À1 ; K 0 = 189 nM) as shown in panel E and described in the text.
Fig. 2 Sequence and single turnover kinetics of MD1 cleavage by E. coli RNase P. (A) Design and sequence of MD1 substrate consisting of two annealed synthetic RNA oligonucleotides.The nucleotides in ptRNA consisting of the stacked acceptor and TCC stem included in MD1 are boxed, and a red arrow indicates the RNase P cleavage site.(B) PAGE analysis of products from a reaction containing 50 nM 5 0 Cy3-MD1 and 1 mM E. coli RNase P. The positions in the gel of the annealed MD1 duplex and the 5 0 fragment generated by RNase P cleavage are shown on the left.Lane M contains equal amounts of the annealed MD1 substrate and a synthetic RNA oligo matching the expected cleavage product (Table 1).(C) Plot of fraction (F) of product formed from total substrate concentration ([P]/([P] + [S])) determined by phosphorimager analysis versus time.These data are fit to an exponential function (eqn (1), Methods) to determine k obs .(D) Dependence of k obs for MD1 single turnover reactions as a function of increasing E. coli RNase P concentration.These data are fit to an equation for Scheme 1 involving equilibrium binding followed by the substrate cleavage step (eqn (2), Methods; k c = 0.017 s À1 ; K 0 = 189 nM) as shown in panel E and described in the text.

Fig. 3
Fig. 3 Analyses of 5 0 2Ap(-2)-MD1 reaction with E. coli RNase P using equilibrium and stopped-flow fluorescence spectroscopy.(A) Equilibrium fluorescence spectra (l ex = 300 nm) of 100 nM 5 0 2Ap(-2)-MD1 (substrate, black line), and 100 nM 5 0 2Ap(-2)-MD1 combined with 1 mM E. coli RNase P in 0.1 M NaCl, 17.5 mM MgCl 2 , 0.1 mM EDTA (product, red line), and 100 nM 5 0 2Ap(-2)-MD1 combined with 1 mM E. coli RNase P, in the same reaction buffer with 17.5 mM CaCl 2 instead of MgCl 2 (ES complex, blue line).(B) Stopped flow fluorescence experiment measuring total fluorescence using a 320 nm high pass filter to measure total fluorescence above the cut off wavelength and excitation at 300 nm using an LED source as described in Methods.Timedependent change in fluorescence in detector voltage upon mixing to achieve final concentrations of 100 nM 5 0 2Ap(-2)-MD1 and 1 mM E. coli RNase P. The data fit a double exponential function (eqn (3), red line) as described in Methods (0.16 s À1 for k obs1 and 0.024 s À1 for k obs2 ).(C) Time-dependent change in fluorescence upon mixing to achieve 100 nM 5 0 2Ap(-2)-MD1 and 1 mM E. coli RNase P in the same reaction buffer with 17.5 mM CaCl 2 instead of MgCl 2 .These data were fit to a single exponential function (eqn (1), k obs = 0.64 s À1 ).(D) Shorter time scale for the same reaction in panel C showing the initial decrease in fluorescence signal.

Fig. 4
Fig. 4 Global fitting determination of k 1 , k À1 , and k 2 for 5 0 Ap(-2)-MD1 cleavage by RNase P. (A) Time-dependent change in fluorescence upon mixing substrate and enzyme to achieve final concentrations of 100 nM 5 0 2Ap(-2)-MD1 and 0.5 mM (black line and data), 0.75 mM (blue line and data), and 1 mM E. coli RNase P (red line and data).The data fit the rate equation for Scheme 1 as described in Methods.(B) Kinetics of the individual changes in S (black), ES (red), and EP (green) for fitting Scheme 1 to the 100 nM 5 0 2Ap(-2)-MD1 and 0.75 mM E. coli RNase P data.(C) Observed dependence of average values for k 1 (black circles), k À1 (red squares), and k 2 (green triangles) for reactions containing 0.5 mM, 0.75 mM, and 1 mM E. coli RNase P. The data are fit to a linear function in order to illustrate reaction order.(D) Summary of k 1 , k À1 , k 2 and K 0 values obtained from global fitting to the kinetic model shown in Scheme 1; values in parentheses were inferred from single turnover kinetics using PAGE analysis.

Fig. 6
Fig. 6 Multiple turnover kinetics of 5 0 Cy3Ap(-2)BHQ-MD1 cleavage by E. coli RNase P. (A) Steady state fluorescence spectra (l ex = 550 nm) of 100 nM 5 0 Cy3Ap(-2)BHQ-MD1 (substrate, black line), and 100 nM 5 0 Cy3Ap(-2)BHQ-MD1 combined with 1 mM E. coli RNase P in 17.5 mM MgCl 2 , (product, red line), or with 1 mM E. coli RNase P in 17.5 mM CaCl 2 (ES complex, blue line).(B) Stopped flow fluorescence experiment measuring total fluorescence using a 570 nm high pass filter and excitation at 535 nm using an LED source as described in Methods.Time-dependent change in fluorescence in detector voltage upon mixing to achieve single turnover conditions with final concentrations of 100 nM 5 0 Cy3Ap(-2)BHQ-MD1 and 1 mM E. coli RNase P. The data were fit to a single exponential function (eqn (1)) where k obs = 0.026 s À1 .(C) Multiple turnover kinetics of Cy3 fluorescence increase upon cleavage measured using plate reader as described in Methods.Time-dependent change in fluorescence intensity upon mixing to achieve final concentrations of 50 nM-5 mM 5 0 Cy3Ap(-2)BHQ-MD1 and 10 nM E. coli RNase P. (D) Kinetics data are fit to saturation binding equation consistent with Scheme 1 to estimate k cat (0.5 s À1 ) and K m (1.8 mM) (eqn (2), Methods).

Fig. 7
Fig. 7 Effects of A248U, G332U, and A333U mutation on E. coli RNase P binding and cleavage kinetics.(A) RNase P active site indicating the positions of the cleavage site between U À1 and G 1 (green), and the active site residues A248, G332, and A333 in P RNA (red), the C5 protein subunit is omitted for clarity.(B) Sequence conservation logo of J18/2 from Type A, Type B, and all seed alignment rnpB gene sequences in the Rfam database.The positions homologous to nucleotides G332 and A333 in E. coli RNase P are highlighted by a dashed box.(C) Denaturing PAGE analysis of the cleavage products of 5 0 Cy3-MD1 for reactions with RNase P and mutants A238U, G332U, and A333U.(D) Plot of k obs for the single turnover reactions of 5 0 Cy3-MD1 with A248U (open circles), G332U (open squares), and A333U (filled triangles).The data fit an equation for the dependence of k obs on [E] according to Scheme 1 as described in Methods (Table2).(E) and (F) stopped flow fluorescence experiment measuring total fluorescence using a 320 nm high pass filter and excitation at 300 nm with an LED source as described in Methods.Time-dependent change in fluorescence in detector voltage upon mixing to achieve final concentrations of 100 nM 5 0 2Ap(-2)-MD1 and 1 mM G332U (E) or A333U (F) mutant RNase P. The data were fit to eqn (3) to estimate k obs2 (i.e.k c ) (G332U k obs2 = 0.023 s À1 , A333U k obs2 = 0.013 s À1 ).

Fig. 8
Fig. 8 Effects of U69A and C70U mutation on E. coli RNase P binding and cleavage kinetics.(A) Analysis of the cleavage products of 5 0 Cy3-MD1 by PAGE for reactions with RNase P mutants U69A and C70U.(B) Plot of k obs for the single turnover reactions of 5 0 -Cy3-MD1 as a function of enzyme concentration: U69A (filled circles), C70U (open circles).The data are fit to eqn (2) for Scheme 1 as described in Methods (Table 1).(C) and (D) Stopped flow fluorescence experiment.2Ap(-2)-MD1 and mutant E. coli RNase P U69A (C) and C70U (D) were mixed to final concentrations of 100 nM and 1 mM, respectively.

Fig. 9
Fig. 9 Differential effects of C70U and U69A mutations on P RNA structure and catalysis in the presence of Mg 2+ versus Ca 2+ .(A) Single turnover kinetics (k 2 ) for native (WT), C70U, and U69A mutant RNase P enzymes in the presence of Mg 2+ or Ca 2+ .The data are shown on a log scale.(B) CryoEM density map and structure model of the active site of E. coli RNase P enzyme-substrate complex (PDB: 7UO5).The positions of G1, A67, G68, and U69 are indicated, the green sphere is an active site metal.(C) SHAPE reactivity analysis of the modification patterns observed for E. coli P RNA in the presence of Mg 2+ versus Ca 2+ .The color of the circles for individual nucleotides reflects the normalized modification score with dark colors indicating higher reactivity.Red/orange circles indicate sites of modification observed in both Mg 2+ and Ca 2+ .Green/light green circles show the sites of modification observed only in Ca 2+ , while the blue/light blue circles indicate the positions detected only in P RNA folded in Mg 2+ .

Table 2
Single turnover kinetic parameters K 0 and k c measured for WT and mutant E. coli RNase P enzymes 57,60 purified from in vitro transcription was incubated at 95 1C for 3 minutes in reaction buffer (MES pH 6 or Tris pH 8; 100 mM NaCl, 0.15% Triton x-100), followedRSC Chemical BiologyPaper by incubated at 37 1C for 10 minutes.MgCl 2 or CaCl 2 was added, and the incubation continued at 37 1C for another 10 minutes.The RNase P holoenzyme was assembled by adding C5 at a ratio of 1 : 1.5 and further reaction for 10 minutes at 37 1C.57,60 obs was determined by plotting the fraction of product formed (y = [P]/([P] + [S])) vs. time (x) and fitting the data to a single exponential function (eqn (1)) in Origin 8.5.The dependence of k obs on [E] was analyzed assuming a rapid equilibrium mechanism (k À1 c k 2 ), using eqn(2), where K 0 is the dissociation constant for MD1 binding to E. coli RNase P, and k c is the first-order rate constant for conversion of ES to EP according to Scheme 1. y = a + be Àkobsx(1)