-
Je něco špatně v tomto záznamu ?
Functional characterization of mutants in the transmembrane domains of the rat P2X7 receptor that regulate pore conductivity and agonist sensitivity
M. Jindrichova, A. Bhattacharya, M. Rupert, P. Skopek, T. Obsil, H. Zemkova,
Jazyk angličtina Země Anglie, Velká Británie
Typ dokumentu časopisecké články, práce podpořená grantem
NLK
Free Medical Journals
od 1997 do Před 1 rokem
Wiley Free Content
od 1997 do Před 1 rokem
PubMed
25712548
DOI
10.1111/jnc.13078
Knihovny.cz E-zdroje
- MeSH
- HEK293 buňky MeSH
- krysa rodu rattus MeSH
- lidé MeSH
- metoda terčíkového zámku MeSH
- molekulární sekvence - údaje MeSH
- mutace MeSH
- mutageneze cílená MeSH
- purinergní receptory P2X7 chemie metabolismus MeSH
- sekvence aminokyselin MeSH
- terciární struktura proteinů MeSH
- transfekce MeSH
- transport proteinů MeSH
- zvířata MeSH
- Check Tag
- krysa rodu rattus MeSH
- lidé MeSH
- zvířata MeSH
- Publikační typ
- časopisecké články MeSH
- práce podpořená grantem MeSH
In the sustained presence of agonist, the opening of P2X7R channel is followed by pore dilatation, which causes an increase in its permeability to larger organic cations, accompanied by receptor sensitization. To explore the molecular mechanisms by which the conductivity and sensitivity are increased, we analyzed the electrophysiological properties and YO-PRO-1 uptake of selected alanine mutants in the first and second transmembrane domains of the rat P2X7R. Substitution of residues Y40, F43, G338, and D352 with alanine reduced membrane trafficking, and the D352A was practically non-functional. The Y40A and F43A mutants that were expressed in the membrane lacked pore dilation ability. Moreover, the Y40A and Y40F displayed desensitization, whereas the Y40W partially recovered receptor function. The G338A/S mutations favored the open state of the channel and displayed instantaneous permeability to larger organic cations. The G338P was non-functional. The L341A and G345A displayed normal trafficking, current amplitude, and sensitization, but both mutations resulted in a decreased pore formation and dye uptake. These results showed that the increase in P2X7R conductivity and sensitivity is critically dependent on residues Y40 and F43 in the TM1 domain and that the region located at the intersection of TM2 helices controls the rate of large pore opening. We investigated the mechanism of the proapoptotic receptor P2X7R's large pore opening and its sensitization. We found that aromatic residues in the upper part of the first transmembrane domain (TM1) are critical for both the P2X7R channel pore opening and receptor sensitization, and residues located at or below the intersection of the second transmembrane domains (TM2) control the rate of pore opening. These findings identify new residues involved in pore formation of P2X7R.
Citace poskytuje Crossref.org
- 000
- 00000naa a2200000 a 4500
- 001
- bmc15031452
- 003
- CZ-PrNML
- 005
- 20151013122847.0
- 007
- ta
- 008
- 151005s2015 enk f 000 0|eng||
- 009
- AR
- 024 7_
- $a 10.1111/jnc.13078 $2 doi
- 035 __
- $a (PubMed)25712548
- 040 __
- $a ABA008 $b cze $d ABA008 $e AACR2
- 041 0_
- $a eng
- 044 __
- $a enk
- 100 1_
- $a Jindrichova, Marie $u Department of Cellular and Molecular Neuroendocrinology, Institute of Physiology of the Academy of Sciences of the Czech Republic, Prague, Czech Republic.
- 245 10
- $a Functional characterization of mutants in the transmembrane domains of the rat P2X7 receptor that regulate pore conductivity and agonist sensitivity / $c M. Jindrichova, A. Bhattacharya, M. Rupert, P. Skopek, T. Obsil, H. Zemkova,
- 520 9_
- $a In the sustained presence of agonist, the opening of P2X7R channel is followed by pore dilatation, which causes an increase in its permeability to larger organic cations, accompanied by receptor sensitization. To explore the molecular mechanisms by which the conductivity and sensitivity are increased, we analyzed the electrophysiological properties and YO-PRO-1 uptake of selected alanine mutants in the first and second transmembrane domains of the rat P2X7R. Substitution of residues Y40, F43, G338, and D352 with alanine reduced membrane trafficking, and the D352A was practically non-functional. The Y40A and F43A mutants that were expressed in the membrane lacked pore dilation ability. Moreover, the Y40A and Y40F displayed desensitization, whereas the Y40W partially recovered receptor function. The G338A/S mutations favored the open state of the channel and displayed instantaneous permeability to larger organic cations. The G338P was non-functional. The L341A and G345A displayed normal trafficking, current amplitude, and sensitization, but both mutations resulted in a decreased pore formation and dye uptake. These results showed that the increase in P2X7R conductivity and sensitivity is critically dependent on residues Y40 and F43 in the TM1 domain and that the region located at the intersection of TM2 helices controls the rate of large pore opening. We investigated the mechanism of the proapoptotic receptor P2X7R's large pore opening and its sensitization. We found that aromatic residues in the upper part of the first transmembrane domain (TM1) are critical for both the P2X7R channel pore opening and receptor sensitization, and residues located at or below the intersection of the second transmembrane domains (TM2) control the rate of pore opening. These findings identify new residues involved in pore formation of P2X7R.
- 650 _2
- $a sekvence aminokyselin $7 D000595
- 650 _2
- $a zvířata $7 D000818
- 650 _2
- $a HEK293 buňky $7 D057809
- 650 _2
- $a lidé $7 D006801
- 650 _2
- $a molekulární sekvence - údaje $7 D008969
- 650 _2
- $a mutageneze cílená $7 D016297
- 650 _2
- $a mutace $7 D009154
- 650 _2
- $a metoda terčíkového zámku $7 D018408
- 650 _2
- $a terciární struktura proteinů $7 D017434
- 650 _2
- $a transport proteinů $7 D021381
- 650 _2
- $a krysa rodu Rattus $7 D051381
- 650 _2
- $a purinergní receptory P2X7 $x chemie $x metabolismus $7 D058486
- 650 _2
- $a transfekce $7 D014162
- 655 _2
- $a časopisecké články $7 D016428
- 655 _2
- $a práce podpořená grantem $7 D013485
- 700 1_
- $a Bhattacharya, Anirban $u Department of Cellular and Molecular Neuroendocrinology, Institute of Physiology of the Academy of Sciences of the Czech Republic, Prague, Czech Republic.
- 700 1_
- $a Rupert, Marian $u Department of Cellular and Molecular Neuroendocrinology, Institute of Physiology of the Academy of Sciences of the Czech Republic, Prague, Czech Republic.
- 700 1_
- $a Skopek, Petr $u Department of Cellular and Molecular Neuroendocrinology, Institute of Physiology of the Academy of Sciences of the Czech Republic, Prague, Czech Republic.
- 700 1_
- $a Obsil, Tomas $u Department of Physical and Macromolecular Chemistry, Faculty of Science, Charles University, Prague, Czech Republic.
- 700 1_
- $a Zemkova, Hana $u Department of Cellular and Molecular Neuroendocrinology, Institute of Physiology of the Academy of Sciences of the Czech Republic, Prague, Czech Republic.
- 773 0_
- $w MED00002832 $t Journal of neurochemistry $x 1471-4159 $g Roč. 133, č. 6 (2015), s. 815-27
- 856 41
- $u https://pubmed.ncbi.nlm.nih.gov/25712548 $y Pubmed
- 910 __
- $a ABA008 $b sig $c sign $y a $z 0
- 990 __
- $a 20151005 $b ABA008
- 991 __
- $a 20151013123036 $b ABA008
- 999 __
- $a ok $b bmc $g 1092328 $s 914578
- BAS __
- $a 3
- BAS __
- $a PreBMC
- BMC __
- $a 2015 $b 133 $c 6 $d 815-27 $e 20150318 $i 1471-4159 $m Journal of neurochemistry $n J Neurochem $x MED00002832
- LZP __
- $a Pubmed-20151005
