Plasma membrane/cytoskeleton interactions in plants

Sonesson, Anders

Plasma membrane/cytoskeleton interactions in plants

Mark

Sonesson, Anders ^LU

(1997)

Abstract: The way in which the cortical cytoskeleton associates to the plasma membrane (PM) must be elucidated to understand the structural dynamics of many processes in the plant cell. In the present study, isolated cauliflower (Brassica oleracea L.) PM vesicles were used to characterize membrane/cytoskeleton interactions. Both actin and tubulin were shown to copurify with PM vesicles and this copurification was specific to the PM. In order to expose the PM-associated cytoskeleton, Brij 58 was used to form sealed, inside-out vesicles (cytoplasmic side out). Both actin and tubulin colocalized with Brij 58-treated PM vesicles in sucrose-gradient centrifugation, indicating a lack of disruption of the actin/PM and tubulin/PM associations following... (More); The way in which the cortical cytoskeleton associates to the plasma membrane (PM) must be elucidated to understand the structural dynamics of many processes in the plant cell. In the present study, isolated cauliflower (Brassica oleracea L.) PM vesicles were used to characterize membrane/cytoskeleton interactions. Both actin and tubulin were shown to copurify with PM vesicles and this copurification was specific to the PM. In order to expose the PM-associated cytoskeleton, Brij 58 was used to form sealed, inside-out vesicles (cytoplasmic side out). Both actin and tubulin colocalized with Brij 58-treated PM vesicles in sucrose-gradient centrifugation, indicating a lack of disruption of the actin/PM and tubulin/PM associations following inside-out vesicle formation. In order to characterize the PM links to actin and tubulin, inside-out PM vesicles were washed in a range of media. Both actin and tubulin co-sedimented with the PM vesicles in the presence of 50 mM DTT, 10 mM CaCl2 and 2 M NaCl (separately). Actin, but not tubulin, was completely released in the presence of 0.6 M KI, and both proteins were released in either 6 M urea or at pH>11.4. The association of actin to the PM was sensitive to extensive dialysis against a low ionic-strength medium. The presence of a pool of a- and b-tubulin with hydrophobic properties, "hydrophobic tubulin", was shown by Triton X-114 fractionation. This hydrophobicity was restricted to PM-associated tubulin and was not seen in soluble tubulin. Hydrophobic tubulin constituted at least 15% of the recovered PM-associated tubulin. Washes in the presence of high concentrations of salt or calcium did not release the hydrophobic tubulin, while high pH (“11.0) did release this fraction. The hydrophobicity of a fraction of the recovered tubulin could reflect a direct or indirect interaction of this tubulin with the PM lipid bilayer or to an integral membrane protein. Hydrophobic tubulin was associated in a salt-sensitive manner to detergent-resistant proteins, likely to be of peripheral/cytoskeletal origin. It is possible that the presence of hydrophobic tubulin in isolated PM reflects the anchoring of the cortical tubulin cytoskeleton to the PM. Further elucidation of the cytoskeleton anchoring mechanism, based on the present study will lead to a better understanding of the structural dynamics of many cellular events. (Less)

Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/29213

author

Sonesson, Anders ^LU

supervisor

Susanne Widell ^LU

opponent

Dr Cyr, Richard J., Department of Biology, The Pennsylvania State University, University Park, Pennsylvania, USA

organization

v1000000

publishing date

1997

type

Thesis

publication status

published

subject

keywords

Triton X-114, hydrophobic tubulin, tubulin, actin, cytoskeleton, Brij 58, inside-out, plasma membrane, plant, cauliflower, Physiological biophysics, Växtfysiologi

pages

105 pages

publisher

Section of Plant Physiology, P.O.Box 117, S-221 00 Lund, Sweden,

defense location

Department of Plant Biology, Sölvegatan 35, Lund

defense date

1997-05-27 10:15:00

external identifiers

other:ISRN: LUNBDS/nbfb-1033/1-105

ISBN

91-628-2529-1

language

English

LU publication?

yes

additional info

The information about affiliations in this record was updated in December 2015. The record was previously connected to the following departments: Biology building (Closed 2011) (011008000), Centre for Educational Development (CED) (018005300), Centre for Teaching and Learning (013100003) Department affilation moved from v1000887 (CED - Centre for Educational Development) to v1000942 (Division for Higher Education Development) on 2016-03-31 08:48:45.

id

ba6c44b4-82e6-4bdc-91ed-731434de94b8 (old id 29213)

date added to LUP

2016-04-04 10:50:28

date last changed

2018-11-21 21:01:04

@phdthesis{ba6c44b4-82e6-4bdc-91ed-731434de94b8,
  abstract     = {{The way in which the cortical cytoskeleton associates to the plasma membrane (PM) must be elucidated to understand the structural dynamics of many processes in the plant cell. In the present study, isolated cauliflower (Brassica oleracea L.) PM vesicles were used to characterize membrane/cytoskeleton interactions. Both actin and tubulin were shown to copurify with PM vesicles and this copurification was specific to the PM. In order to expose the PM-associated cytoskeleton, Brij 58 was used to form sealed, inside-out vesicles (cytoplasmic side out). Both actin and tubulin colocalized with Brij 58-treated PM vesicles in sucrose-gradient centrifugation, indicating a lack of disruption of the actin/PM and tubulin/PM associations following inside-out vesicle formation. In order to characterize the PM links to actin and tubulin, inside-out PM vesicles were washed in a range of media. Both actin and tubulin co-sedimented with the PM vesicles in the presence of 50 mM DTT, 10 mM CaCl2 and 2 M NaCl (separately). Actin, but not tubulin, was completely released in the presence of 0.6 M KI, and both proteins were released in either 6 M urea or at pH&gt;11.4. The association of actin to the PM was sensitive to extensive dialysis against a low ionic-strength medium. The presence of a pool of a- and b-tubulin with hydrophobic properties, "hydrophobic tubulin", was shown by Triton X-114 fractionation. This hydrophobicity was restricted to PM-associated tubulin and was not seen in soluble tubulin. Hydrophobic tubulin constituted at least 15% of the recovered PM-associated tubulin. Washes in the presence of high concentrations of salt or calcium did not release the hydrophobic tubulin, while high pH (“11.0) did release this fraction. The hydrophobicity of a fraction of the recovered tubulin could reflect a direct or indirect interaction of this tubulin with the PM lipid bilayer or to an integral membrane protein. Hydrophobic tubulin was associated in a salt-sensitive manner to detergent-resistant proteins, likely to be of peripheral/cytoskeletal origin. It is possible that the presence of hydrophobic tubulin in isolated PM reflects the anchoring of the cortical tubulin cytoskeleton to the PM. Further elucidation of the cytoskeleton anchoring mechanism, based on the present study will lead to a better understanding of the structural dynamics of many cellular events.}},
  author       = {{Sonesson, Anders}},
  isbn         = {{91-628-2529-1}},
  keywords     = {{Triton X-114; hydrophobic tubulin; tubulin; actin; cytoskeleton; Brij 58; inside-out; plasma membrane; plant; cauliflower; Physiological biophysics; Växtfysiologi}},
  language     = {{eng}},
  publisher    = {{Section of Plant Physiology, P.O.Box 117, S-221 00 Lund, Sweden,}},
  school       = {{Lund University}},
  title        = {{Plasma membrane/cytoskeleton interactions in plants}},
  year         = {{1997}},
}

Lund University Publications

LUND UNIVERSITY LIBRARIES

Plasma membrane/cytoskeleton interactions in plants