Identification of phosphatidate nonlamellar phases on liposomes by flow cytometry.

I. Baeza; L. Aguilar; F. Alvarado-Alemán; C. Soto; A. Escobar-Gutiérrez; R. Mondragón; S. González; M. Ibáñez; C. Wong

doi:10.1139/o95-036

Identification of phosphatidate nonlamellar phases on liposomes by flow cytometry.

I. Baeza, L. Aguilar, F. Alvarado-Alemán, C. Soto, A. Escobar-Gutiérrez, R. Mondragón, S. González, M. Ibáñez, C. Wong

Research output: Contribution to journal › Article › peer-review

6 Scopus citations

Abstract

This study is the first report that demonstrates nonlamellar arrangements, or lipidic particles, of phosphatidate inserted in the lipid bilayer of liposomes using polyclonal antibodies from mice and flow cytometry. Sera immunoreactivity was analyzed using liposomes that displayed smooth bilayers of phosphatidate particles, as shown by electron microscopy. This cytofluorimetric analysis showed that immune mice sera have a specific immunoreactivity with the phosphatide particles formed by Mn2+, which also cross-reacted with those formed by Ca2+ and with cardiolipin particles formed by Mn2+. In addition, these immune sera hardly reacted with smooth bilayered liposomes, independently of the lipid composition studied. Thus, this new methodology can be applied to demonstrate nonlamellar molecular arrangements in biological membranes.

Original language	English
Pages (from-to)	289-297
Number of pages	9
Journal	Biochemistry and Cell Biology
Volume	73
Issue number	5-6
DOIs	https://doi.org/10.1139/o95-036
State	Published - 1995

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title = "Identification of phosphatidate nonlamellar phases on liposomes by flow cytometry.",

abstract = "This study is the first report that demonstrates nonlamellar arrangements, or lipidic particles, of phosphatidate inserted in the lipid bilayer of liposomes using polyclonal antibodies from mice and flow cytometry. Sera immunoreactivity was analyzed using liposomes that displayed smooth bilayers of phosphatidate particles, as shown by electron microscopy. This cytofluorimetric analysis showed that immune mice sera have a specific immunoreactivity with the phosphatide particles formed by Mn2+, which also cross-reacted with those formed by Ca2+ and with cardiolipin particles formed by Mn2+. In addition, these immune sera hardly reacted with smooth bilayered liposomes, independently of the lipid composition studied. Thus, this new methodology can be applied to demonstrate nonlamellar molecular arrangements in biological membranes.",

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doi = "10.1139/o95-036",

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T1 - Identification of phosphatidate nonlamellar phases on liposomes by flow cytometry.

AU - Baeza, I.

AU - Aguilar, L.

AU - Alvarado-Alemán, F.

AU - Soto, C.

AU - Escobar-Gutiérrez, A.

AU - Mondragón, R.

AU - González, S.

AU - Ibáñez, M.

AU - Wong, C.

PY - 1995

Y1 - 1995

N2 - This study is the first report that demonstrates nonlamellar arrangements, or lipidic particles, of phosphatidate inserted in the lipid bilayer of liposomes using polyclonal antibodies from mice and flow cytometry. Sera immunoreactivity was analyzed using liposomes that displayed smooth bilayers of phosphatidate particles, as shown by electron microscopy. This cytofluorimetric analysis showed that immune mice sera have a specific immunoreactivity with the phosphatide particles formed by Mn2+, which also cross-reacted with those formed by Ca2+ and with cardiolipin particles formed by Mn2+. In addition, these immune sera hardly reacted with smooth bilayered liposomes, independently of the lipid composition studied. Thus, this new methodology can be applied to demonstrate nonlamellar molecular arrangements in biological membranes.

AB - This study is the first report that demonstrates nonlamellar arrangements, or lipidic particles, of phosphatidate inserted in the lipid bilayer of liposomes using polyclonal antibodies from mice and flow cytometry. Sera immunoreactivity was analyzed using liposomes that displayed smooth bilayers of phosphatidate particles, as shown by electron microscopy. This cytofluorimetric analysis showed that immune mice sera have a specific immunoreactivity with the phosphatide particles formed by Mn2+, which also cross-reacted with those formed by Ca2+ and with cardiolipin particles formed by Mn2+. In addition, these immune sera hardly reacted with smooth bilayered liposomes, independently of the lipid composition studied. Thus, this new methodology can be applied to demonstrate nonlamellar molecular arrangements in biological membranes.

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U2 - 10.1139/o95-036

DO - 10.1139/o95-036

M3 - Artículo

SN - 0829-8211

VL - 73

SP - 289

EP - 297

JO - Biochemistry and Cell Biology

JF - Biochemistry and Cell Biology

IS - 5-6

ER -

Identification of phosphatidate nonlamellar phases on liposomes by flow cytometry.

Abstract

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