Comparative analysis of widely used methods to remove nonfunctional myosin heads for the in vitro motility assay

Rahman, Mohammad A.; Salhotra, Aseem; Månsson, Alf

doi:10.1007/s10974-019-09505-1

Cited by 18 publications

(15 citation statements)

References 52 publications

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“…Second, the independence between experimental occasions and myosin batch is supported by our data in Supplementary Figs. 16, 18 as well as previous data showing very similar kinetic properties of myosin from different preparations 76 , 102 . Accordingly, we found similar results in three hs-AFM experiments performed on different days using different surface preparations, solutions and HMM from two different myosin preparations.…”

Section: Methodssupporting

confidence: 76%

“…In the replication of single-molecule fluorescence experiments, each binding event of a fluorescent ATP molecule to a myosin molecule was assumed to be an independent random event independent of the experimental occasion, or myosin batch as supported by previous findings of very similar kinetic properties of myosin from different preparations 76 , 102 . Furthermore, the assumption is supported by similar results in experiments performed on different days and/or using different myosin preparations (Fig.…”

Section: Methodsmentioning

confidence: 99%

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Multistep orthophosphate release tunes actomyosin energy transduction

et al. 2022

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Muscle contraction and a range of critical cellular functions rely on force-producing interactions between myosin motors and actin filaments, powered by turnover of adenosine triphosphate (ATP). The relationship between release of the ATP hydrolysis product ortophosphate (Pi) from the myosin active site and the force-generating structural change, the power-stroke, remains enigmatic despite its central role in energy transduction. Here, we present a model with multistep Pi-release that unifies current conflicting views while also revealing additional complexities of potential functional importance. The model is based on our evidence from kinetics, molecular modelling and single molecule fluorescence studies of Pi binding outside the active site. It is also consistent with high-speed atomic force microscopy movies of single myosin II molecules without Pi at the active site, showing consecutive snapshots of pre- and post-power stroke conformations. In addition to revealing critical features of energy transduction by actomyosin, the results suggest enzymatic mechanisms of potentially general relevance.

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Section: Methodssupporting

confidence: 76%

Section: Methodsmentioning

confidence: 99%

Multistep orthophosphate release tunes actomyosin energy transduction

et al. 2022

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“…No sample size calculation was performed prior to the experiments. Instead we relied on previous information 7 , 80 .…”

Section: Methodsmentioning

confidence: 99%

Single molecule turnover of fluorescent ATP by myosin and actomyosin unveil elusive enzymatic mechanisms

et al. 2021

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Benefits of single molecule studies of biomolecules include the need for minimal amounts of material and the potential to reveal phenomena hidden in ensembles. However, results from recent single molecule studies of fluorescent ATP turnover by myosin are difficult to reconcile with ensemble studies. We found that key reasons are complexities due to dye photophysics and fluorescent contaminants. After eliminating these, through surface cleaning and use of triple state quenchers and redox agents, the distributions of ATP binding dwell times on myosin are best described by 2 to 3 exponential processes, with and without actin, and with and without the inhibitor para-aminoblebbistatin. Two processes are attributable to ATP turnover by myosin and actomyosin respectively, whereas the remaining process (rate constant 0.2–0.5 s−1) is consistent with non-specific ATP binding to myosin, possibly accelerating ATP transport to the active site. Finally, our study of actin-activated myosin ATP turnover without sliding between actin and myosin reveals heterogeneity in the ATP turnover kinetics consistent with models of isometric contraction.

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“…Finally, assay solution was prepared by adding 0.2 mg mL À1 creatine phosphokinase (CPK), 2.5 mM creatine phosphate (CP), 1 mM magnesium adenosine triphosphate (MgATP), an oxygen scavenger mixture (GOC): 3 mg mL À1 glucose : 0.1 mg mL À1 glucose oxidase, 0.02 mg mL À1 catalase, 10 mM DTT, and 45 mM (KCl) to the LISS solution, giving a final ionic strength of 60 mM. [45,46] In Vitro Motility Assays: HMM, fluorescently labeled actin and nonfluorescent-blocking actin, [47] were diluted in the wash solution. To perform the in vitro motility assay, flow cells were built using a glass coverslip and a nanostructured chip on top, separated with Parafilm spacers.…”

Section: Methodsmentioning

confidence: 99%

Solving the 3‐Satisfiability Problem Using Network‐Based Biocomputation

Zhu

Salhotra

Meinecke

et al. 2022

Advanced Intelligent Systems

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The 3‐satisfiability Problem (3‐SAT) is a demanding combinatorial problem that is of central importance among the nondeterministic polynomial (NP) complete problems, with applications in circuit design, artificial intelligence, and logistics. Even with optimized algorithms, the solution space that needs to be explored grows exponentially with the increasing size of 3‐SAT instances. Thus, large 3‐SAT instances require excessive amounts of energy to solve with serial electronic computers. Network‐based biocomputation (NBC) is a parallel computation approach with drastically reduced energy consumption. NBC uses biomolecular motors to propel cytoskeletal filaments through nanofabricated networks that encode mathematical problems. By stochastically exploring possible paths through the networks, the cytoskeletal filaments find possible solutions. However, to date, no NBC algorithm for 3‐SAT has been available. Herein, an algorithm that converts 3‐SAT into an NBC‐compatible network format is reported and four small 3‐SAT instances (with up to three variables and five clauses) using the actin–myosin biomolecular motor system are experimentally solved. Because practical polynomial conversions to 3‐SAT exist for many important NP complete problems, the result opens the door to enable NBC to solve small instances of a wide range of problems.

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Comparative analysis of widely used methods to remove nonfunctional myosin heads for the in vitro motility assay

Cited by 18 publications

References 52 publications

Multistep orthophosphate release tunes actomyosin energy transduction

Multistep orthophosphate release tunes actomyosin energy transduction

Single molecule turnover of fluorescent ATP by myosin and actomyosin unveil elusive enzymatic mechanisms

Solving the 3‐Satisfiability Problem Using Network‐Based Biocomputation

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