Structure and post-translational modifications of the web silk protein spidroin-1 from Nephila spiders

José Roberto Aparecido dos Santos-Pinto; Günther Lamprecht; Wei Qiang Chen; Seok Heo; John George Hardy; Helga Priewalder; Thomas Rainer Scheibel; Mario Sergio Palma; Gert Lubec

doi:10.1016/j.jprot.2014.01.002

Structure and post-translational modifications of the web silk protein spidroin-1 from Nephila spiders

José Roberto Aparecido dos Santos-Pinto, Günther Lamprecht, Wei Qiang Chen, Seok Heo, John George Hardy, Helga Priewalder, Thomas Rainer Scheibel, Mario Sergio Palma, Gert Lubec

Research output: Contribution to journal › Review article › peer-review

28 Scopus citations

Abstract

Spidroin-1 is one of the major ampullate silk proteins produced by spiders for use in the construction of the frame and radii of orb webs, and as a dragline to escape from predators. Only partial sequences of spidroin-1 produced by Nephila clavipes have been reported up to now, and there is no information on post-translational modifications (PTMs). A gel-based mass spectrometry strategy with ETD and CID fragmentation methods were used to sequence and determine the presence/location of any PTMs on the spidroin-1. Sequence coverage of 98.06%, 95.05%, and 98.37% were obtained for N. clavipes, Nephila edulis and for Nephila madagascariensis, respectively. Phosphorylation was the major PTM observed with 8 phosphorylation sites considered reliable on spidroin-1 produced by N. clavipes, 4 in N. madagascariensis and 2 for N. edulis. Dityrosine and 3,4-dihydroxyphenylalanine (formed by oxidation of the spidroin-1) were observed, although the mechanism by which they are formed (i.e. exposure to UV radiation or to peroxidases in the major ampullate silk gland) is uncertain. Herein we present structural information on the spidroin-1 produced by three different Nephila species; these findings may be valuable for understanding the physicochemical properties of the silk proteins and moreover, future designs of recombinantly produced spider silk proteins. Biotechnological significance. The present investigation shows for the first time spidroin structure and post-translational modifications observed on the major ampullate silk spidroin-1. The many site specific phosphorylations (localized within the structural motifs) along with the probably photoinduction of hydroxylations may be relevant for scientists in material science, biology, biochemistry and environmental scientists. Up to now all the mechanical properties of the spidroin have been characterized without any consideration about the existence of PTMs in the sequence of spidroins. Thus, these findings for major ampullate silk spidroin-1 from Nephila spiders provide the basis for mechanical-elastic property studies of silk for biotechnological and biomedical potential applications. This article is part of a Special Issue entitled: Proteomics of non-model organisms.

Original language	English (US)
Pages (from-to)	174-185
Number of pages	12
Journal	Journal of Proteomics
Volume	105
DOIs	https://doi.org/10.1016/j.jprot.2014.01.002
State	Published - Jun 13 2014
Externally published	Yes

Keywords

Dityrosine
Mass spectrometry
Peptide sequencing
Phosphorylation
Proteomic analysis

ASJC Scopus subject areas

Biophysics
Biochemistry

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10.1016/j.jprot.2014.01.002

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@article{a11a1338b56a4d8abe71f49f8e2eca8e,

title = "Structure and post-translational modifications of the web silk protein spidroin-1 from Nephila spiders",

abstract = "Spidroin-1 is one of the major ampullate silk proteins produced by spiders for use in the construction of the frame and radii of orb webs, and as a dragline to escape from predators. Only partial sequences of spidroin-1 produced by Nephila clavipes have been reported up to now, and there is no information on post-translational modifications (PTMs). A gel-based mass spectrometry strategy with ETD and CID fragmentation methods were used to sequence and determine the presence/location of any PTMs on the spidroin-1. Sequence coverage of 98.06%, 95.05%, and 98.37% were obtained for N. clavipes, Nephila edulis and for Nephila madagascariensis, respectively. Phosphorylation was the major PTM observed with 8 phosphorylation sites considered reliable on spidroin-1 produced by N. clavipes, 4 in N. madagascariensis and 2 for N. edulis. Dityrosine and 3,4-dihydroxyphenylalanine (formed by oxidation of the spidroin-1) were observed, although the mechanism by which they are formed (i.e. exposure to UV radiation or to peroxidases in the major ampullate silk gland) is uncertain. Herein we present structural information on the spidroin-1 produced by three different Nephila species; these findings may be valuable for understanding the physicochemical properties of the silk proteins and moreover, future designs of recombinantly produced spider silk proteins. Biotechnological significance. The present investigation shows for the first time spidroin structure and post-translational modifications observed on the major ampullate silk spidroin-1. The many site specific phosphorylations (localized within the structural motifs) along with the probably photoinduction of hydroxylations may be relevant for scientists in material science, biology, biochemistry and environmental scientists. Up to now all the mechanical properties of the spidroin have been characterized without any consideration about the existence of PTMs in the sequence of spidroins. Thus, these findings for major ampullate silk spidroin-1 from Nephila spiders provide the basis for mechanical-elastic property studies of silk for biotechnological and biomedical potential applications. This article is part of a Special Issue entitled: Proteomics of non-model organisms.",

keywords = "Dityrosine, Mass spectrometry, Peptide sequencing, Phosphorylation, Proteomic analysis",

author = "{dos Santos-Pinto}, {Jos{\'e} Roberto Aparecido} and G{\"u}nther Lamprecht and Chen, {Wei Qiang} and Seok Heo and Hardy, {John George} and Helga Priewalder and Scheibel, {Thomas Rainer} and Palma, {Mario Sergio} and Gert Lubec",

note = "Funding Information: This work was supported partially by grants from FAPESP ( Proc. 2010/19051-6 and Proc. 2011/51684-1 ), the CNPq and the Gert Lubec Proteomics Laboratory at the University of Vienna . M.S.P. is a researcher from the National Research Council of Brazil—CNPq, provided N. clavipes samples and participated in the original design of the study. J.R.A.S.P. is a PhD student fellow from FAPESP who carried out all analytical work in the Gert Lubec Proteomics Laboratory at the University of Vienna and participated in writing the manuscript. W.Q.C. and S.H. assisted in carrying out analytical work. J.G.H. initiated the collaboration between the Scheibel and Lubec groups, sourced N. edulis and N. madagascariensis samples, assisted in writing the manuscript, and thanks the Alexander Von Humboldt Foundation for a Postdoctoral Research Fellowship. H.P. carried out scanning microscopical analyses. T.R.S. approved the manuscript and thanks both the German Research Foundation (Deutsche Forschungsgemeinschaft, DFG SCHE 603/4-3) and the German Federal Ministry of Education and Research (Bundesministerium f{\"u}r Bildung und Forschung, BMBF 13 N9736) for financial support. G. Lamprecht analyzed tyrosine adducts by HPLC. G. Lubec had the project idea, designed and supervised the study and wrote the manuscript. ",

year = "2014",

month = jun,

day = "13",

doi = "10.1016/j.jprot.2014.01.002",

language = "English (US)",

volume = "105",

pages = "174--185",

journal = "Journal of Proteomics",

issn = "1874-3919",

publisher = "Elsevier B.V.",

}

TY - JOUR

T1 - Structure and post-translational modifications of the web silk protein spidroin-1 from Nephila spiders

AU - dos Santos-Pinto, José Roberto Aparecido

AU - Lamprecht, Günther

AU - Chen, Wei Qiang

AU - Heo, Seok

AU - Hardy, John George

AU - Priewalder, Helga

AU - Scheibel, Thomas Rainer

AU - Palma, Mario Sergio

AU - Lubec, Gert

N1 - Funding Information: This work was supported partially by grants from FAPESP ( Proc. 2010/19051-6 and Proc. 2011/51684-1 ), the CNPq and the Gert Lubec Proteomics Laboratory at the University of Vienna . M.S.P. is a researcher from the National Research Council of Brazil—CNPq, provided N. clavipes samples and participated in the original design of the study. J.R.A.S.P. is a PhD student fellow from FAPESP who carried out all analytical work in the Gert Lubec Proteomics Laboratory at the University of Vienna and participated in writing the manuscript. W.Q.C. and S.H. assisted in carrying out analytical work. J.G.H. initiated the collaboration between the Scheibel and Lubec groups, sourced N. edulis and N. madagascariensis samples, assisted in writing the manuscript, and thanks the Alexander Von Humboldt Foundation for a Postdoctoral Research Fellowship. H.P. carried out scanning microscopical analyses. T.R.S. approved the manuscript and thanks both the German Research Foundation (Deutsche Forschungsgemeinschaft, DFG SCHE 603/4-3) and the German Federal Ministry of Education and Research (Bundesministerium für Bildung und Forschung, BMBF 13 N9736) for financial support. G. Lamprecht analyzed tyrosine adducts by HPLC. G. Lubec had the project idea, designed and supervised the study and wrote the manuscript.

PY - 2014/6/13

Y1 - 2014/6/13

N2 - Spidroin-1 is one of the major ampullate silk proteins produced by spiders for use in the construction of the frame and radii of orb webs, and as a dragline to escape from predators. Only partial sequences of spidroin-1 produced by Nephila clavipes have been reported up to now, and there is no information on post-translational modifications (PTMs). A gel-based mass spectrometry strategy with ETD and CID fragmentation methods were used to sequence and determine the presence/location of any PTMs on the spidroin-1. Sequence coverage of 98.06%, 95.05%, and 98.37% were obtained for N. clavipes, Nephila edulis and for Nephila madagascariensis, respectively. Phosphorylation was the major PTM observed with 8 phosphorylation sites considered reliable on spidroin-1 produced by N. clavipes, 4 in N. madagascariensis and 2 for N. edulis. Dityrosine and 3,4-dihydroxyphenylalanine (formed by oxidation of the spidroin-1) were observed, although the mechanism by which they are formed (i.e. exposure to UV radiation or to peroxidases in the major ampullate silk gland) is uncertain. Herein we present structural information on the spidroin-1 produced by three different Nephila species; these findings may be valuable for understanding the physicochemical properties of the silk proteins and moreover, future designs of recombinantly produced spider silk proteins. Biotechnological significance. The present investigation shows for the first time spidroin structure and post-translational modifications observed on the major ampullate silk spidroin-1. The many site specific phosphorylations (localized within the structural motifs) along with the probably photoinduction of hydroxylations may be relevant for scientists in material science, biology, biochemistry and environmental scientists. Up to now all the mechanical properties of the spidroin have been characterized without any consideration about the existence of PTMs in the sequence of spidroins. Thus, these findings for major ampullate silk spidroin-1 from Nephila spiders provide the basis for mechanical-elastic property studies of silk for biotechnological and biomedical potential applications. This article is part of a Special Issue entitled: Proteomics of non-model organisms.

AB - Spidroin-1 is one of the major ampullate silk proteins produced by spiders for use in the construction of the frame and radii of orb webs, and as a dragline to escape from predators. Only partial sequences of spidroin-1 produced by Nephila clavipes have been reported up to now, and there is no information on post-translational modifications (PTMs). A gel-based mass spectrometry strategy with ETD and CID fragmentation methods were used to sequence and determine the presence/location of any PTMs on the spidroin-1. Sequence coverage of 98.06%, 95.05%, and 98.37% were obtained for N. clavipes, Nephila edulis and for Nephila madagascariensis, respectively. Phosphorylation was the major PTM observed with 8 phosphorylation sites considered reliable on spidroin-1 produced by N. clavipes, 4 in N. madagascariensis and 2 for N. edulis. Dityrosine and 3,4-dihydroxyphenylalanine (formed by oxidation of the spidroin-1) were observed, although the mechanism by which they are formed (i.e. exposure to UV radiation or to peroxidases in the major ampullate silk gland) is uncertain. Herein we present structural information on the spidroin-1 produced by three different Nephila species; these findings may be valuable for understanding the physicochemical properties of the silk proteins and moreover, future designs of recombinantly produced spider silk proteins. Biotechnological significance. The present investigation shows for the first time spidroin structure and post-translational modifications observed on the major ampullate silk spidroin-1. The many site specific phosphorylations (localized within the structural motifs) along with the probably photoinduction of hydroxylations may be relevant for scientists in material science, biology, biochemistry and environmental scientists. Up to now all the mechanical properties of the spidroin have been characterized without any consideration about the existence of PTMs in the sequence of spidroins. Thus, these findings for major ampullate silk spidroin-1 from Nephila spiders provide the basis for mechanical-elastic property studies of silk for biotechnological and biomedical potential applications. This article is part of a Special Issue entitled: Proteomics of non-model organisms.

KW - Dityrosine

KW - Mass spectrometry

KW - Peptide sequencing

KW - Phosphorylation

KW - Proteomic analysis

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U2 - 10.1016/j.jprot.2014.01.002

DO - 10.1016/j.jprot.2014.01.002

M3 - Review article

C2 - 24434585

AN - SCOPUS:84901841295

SN - 1874-3919

VL - 105

SP - 174

EP - 185

JO - Journal of Proteomics

JF - Journal of Proteomics

ER -

Structure and post-translational modifications of the web silk protein spidroin-1 from Nephila spiders

Abstract

Keywords

ASJC Scopus subject areas

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