4.1 Article

Spin Labeling of Surface Cysteines Using a Bromoacrylaldehyde Spin Label

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APPLIED MAGNETIC RESONANCE
卷 52, 期 8, 页码 959-970

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SPRINGER WIEN
DOI: 10.1007/s00723-021-01350-1

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资金

  1. Medical Research Council [MR/K011049/1]
  2. BBSRC DTP Studentship
  3. EPSRC DTA studentship

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This study introduces a new cysteine spin label, BASL, which demonstrates advantages over the traditional MTSSL in terms of selectivity and applicability to multidomain proteins. The use of BASL allows for selective labeling and easy addition in excess, avoiding protein precipitation issues seen with MTSSL, making it a promising candidate for protein binding and in-cell studies. Additionally, DEER spectroscopy with BASL enables precise measurement of distances between cysteine pairs within proteins, showcasing its potential for structural investigations.
Structural investigations of proteins and their biological complexes are now frequently complemented by distance constraints between spin labeled cysteines generated using double electron-electron resonance (DEER) spectroscopy, via site directed spin labeling (SDSL). Methanethiosulfonate spin label (MTSSL), has become ubiquitous in the SDSL of proteins, however, has limitations owing to its high number of rotamers, and reducibility. In this article we introduce the use of bromoacrylaldehyde spin label (BASL) as a cysteine spin label, demonstrating an advantage over MTSSL due to its increased selectivity for surface cysteines, eliminating the need to 'knock out' superfluous cysteine residues. Applied to the multidomain protein, His domain protein tyrosine phosphatase (HD-PTP), we show that BASL can be easily added in excess with selective labeling, whereas MTSSL causes protein precipitation. Furthermore, using DEER, we were able to measure a single cysteine pair distance in a three cysteine domain within HD-PTP. The label has a further advantage of comprising a sulfide in a three-bond tether, making it a candidate for protein binding and in-cell studies.

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