Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluation

To facilitate further evaluation of pheromone biosynthesis activating neuropeptide receptor (PBANR) functionality and regulation, we generated cultured insect cell lines constitutively expressing green fluorescent protein chimeras of the recently identified Bombyx mori PBANR (BommoPBANR) and Pseudal...

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Main Authors: Jae Min Lee, J. Joe Hull, Takeshi eKawai, Kazuhide eTsuneizumi, Masaaki eKuriharaa, Masaru eTanokura, Koji eNagata, Hiromichi eNagasawa, Shogo eMatsumoto
Format: Article
Language:English
Published: Frontiers Media S.A. 2012-04-01
Series:Frontiers in Endocrinology
Subjects:
Online Access:http://journal.frontiersin.org/Journal/10.3389/fendo.2012.00056/full
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spelling doaj-660ad8cf9a3642428c498fdf2ca519b22020-11-25T00:32:10ZengFrontiers Media S.A.Frontiers in Endocrinology1664-23922012-04-01310.3389/fendo.2012.0005621304Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluationJae Min Lee0J. Joe Hull1Takeshi eKawai2Kazuhide eTsuneizumi3Masaaki eKuriharaa4Masaru eTanokura5Koji eNagata6Hiromichi eNagasawa7Shogo eMatsumoto8RIKEN Advanced Science InstituteUSDA Agricultural Research ServiceThe University of TokyoRIKEN Advanced Science InstituteRIKEN Advanced Science InstituteThe University of TokyoThe University of TokyoThe University of TokyoRIKEN Advanced Science InstituteTo facilitate further evaluation of pheromone biosynthesis activating neuropeptide receptor (PBANR) functionality and regulation, we generated cultured insect cell lines constitutively expressing green fluorescent protein chimeras of the recently identified Bombyx mori PBANR (BommoPBANR) and Pseudaletia separata PBANR (PsesePBANR) variants. Fluorescent chimeras included the BommoPBANR-A, B, and C variants and the PsesePBANR-B and C variants. Cell lines expressing non-chimeric BommoPBANR-B and C variants were also generated. Functional evaluation of these transformed cell lines using confocal laser microscopy revealed that a Rhodamine Red-labeled PBAN derivative (RR-C10PBANR2K) specifically co-localized with all of the respective PBANR variants at the plasma membrane. Near complete internalization of the fluorescent RR-C10PBANR2K ligand 30 min after binding was observed in all cell lines except those expressing the BommoPBANR-A variant, in which the ligand/receptor complex remained at the plasma membrane. Fluorescent Ca2+ imaging further showed that, unlike the BommoPBANR-B or BommoPBANR-C cell lines, RR-C10PBANR2K binding failed to mobilize extracellular Ca2+ in the BommoPBANR-A cell line even at concentrations of 10 M. These observations demonstrate a clear functional difference between the BommoPBANR-A variant and the BommoPBANR-B and –C variants in terms of receptor regulation and activation of downstream effector molecules. We also found that, contrary to previous reports, ligand-induced internalization of BommoPBANR-B and BommoPBANR-C in cell lines stably expressing these variants occurred in the absence of extracellular Ca2+.http://journal.frontiersin.org/Journal/10.3389/fendo.2012.00056/fullGPCRCa2+ influxligand-induced internalizationPBAN receptorsplice variantsstable transformation
collection DOAJ
language English
format Article
sources DOAJ
author Jae Min Lee
J. Joe Hull
Takeshi eKawai
Kazuhide eTsuneizumi
Masaaki eKuriharaa
Masaru eTanokura
Koji eNagata
Hiromichi eNagasawa
Shogo eMatsumoto
spellingShingle Jae Min Lee
J. Joe Hull
Takeshi eKawai
Kazuhide eTsuneizumi
Masaaki eKuriharaa
Masaru eTanokura
Koji eNagata
Hiromichi eNagasawa
Shogo eMatsumoto
Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluation
Frontiers in Endocrinology
GPCR
Ca2+ influx
ligand-induced internalization
PBAN receptor
splice variants
stable transformation
author_facet Jae Min Lee
J. Joe Hull
Takeshi eKawai
Kazuhide eTsuneizumi
Masaaki eKuriharaa
Masaru eTanokura
Koji eNagata
Hiromichi eNagasawa
Shogo eMatsumoto
author_sort Jae Min Lee
title Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluation
title_short Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluation
title_full Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluation
title_fullStr Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluation
title_full_unstemmed Establishment of Sf9 transformants constitutively expressing PBAN receptor (PBANR) variants: application to functional evaluation
title_sort establishment of sf9 transformants constitutively expressing pban receptor (pbanr) variants: application to functional evaluation
publisher Frontiers Media S.A.
series Frontiers in Endocrinology
issn 1664-2392
publishDate 2012-04-01
description To facilitate further evaluation of pheromone biosynthesis activating neuropeptide receptor (PBANR) functionality and regulation, we generated cultured insect cell lines constitutively expressing green fluorescent protein chimeras of the recently identified Bombyx mori PBANR (BommoPBANR) and Pseudaletia separata PBANR (PsesePBANR) variants. Fluorescent chimeras included the BommoPBANR-A, B, and C variants and the PsesePBANR-B and C variants. Cell lines expressing non-chimeric BommoPBANR-B and C variants were also generated. Functional evaluation of these transformed cell lines using confocal laser microscopy revealed that a Rhodamine Red-labeled PBAN derivative (RR-C10PBANR2K) specifically co-localized with all of the respective PBANR variants at the plasma membrane. Near complete internalization of the fluorescent RR-C10PBANR2K ligand 30 min after binding was observed in all cell lines except those expressing the BommoPBANR-A variant, in which the ligand/receptor complex remained at the plasma membrane. Fluorescent Ca2+ imaging further showed that, unlike the BommoPBANR-B or BommoPBANR-C cell lines, RR-C10PBANR2K binding failed to mobilize extracellular Ca2+ in the BommoPBANR-A cell line even at concentrations of 10 M. These observations demonstrate a clear functional difference between the BommoPBANR-A variant and the BommoPBANR-B and –C variants in terms of receptor regulation and activation of downstream effector molecules. We also found that, contrary to previous reports, ligand-induced internalization of BommoPBANR-B and BommoPBANR-C in cell lines stably expressing these variants occurred in the absence of extracellular Ca2+.
topic GPCR
Ca2+ influx
ligand-induced internalization
PBAN receptor
splice variants
stable transformation
url http://journal.frontiersin.org/Journal/10.3389/fendo.2012.00056/full
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