Linkage Analysis Using Platelet-activating Factor Ca2+
Response in Transformed Lymphoblasts
L.M. Brzustowicz, J.P. Gardner, L. Hopp, E. Jeanclos, J. Ott,
X.Y. Yang, Z. Fekete, A. Aviv
Hypertension, 29(1 Pt 2), 158-164 (Jan 1997).
Abstract
Epstein-Barr virus-transformed lymphoblasts from patients with
essential hypertension demonstrate enhanced G protein-mediated
cytosolic free calcium (ÍCa2+Íi) response to platelet-activating
factor (PAF). To map genes responsible for variation in G
protein-coupled signaling, we used this cellular phenotype for a
linkage study of transformed cell lines from the Centre d'Etude du
Polymorphisme Humain (CEPH) reference pedigrees. The
PAF-evoked change in ÍCa2+Íi ranged from 20 to 392 mmol/L and
was highly reproducible within each cell line. PAF-elicited ÍCa2+Íi
responses were obtained in lymphoblastic cell lines from five densely
mapped pedigrees of the CEPH collection. Using PAF-evoked
ÍCa2+Íi responses as a quantitative trait, two-point sibpair linkage
analyses were conducted using 5150 markers from the Collaborative
Human Linkage Center (CHLC) database. Nine loci, located on
chromosomes 1, 4, 10, 11, 13, 16, and 17, were suggestive of linkage,
with values of P < 7.4 x 10(-4). Multipoint linkage analysis
produced a significant linkage finding (P = 2.1 x 10(-5) in one
family at D16S151, with suggestive linkage results for seven
additional markers spanning a 40-cM interval of chromosome 16.
Multipoint analysis produced suggestive findings of linkage to eight
loci from two distinct regions of chromosome 11 in another family.
These results indicate that loci involved in the control of G
protein-mediated mechanisms, suggested to be involved in the
pathophysiology of essential hypertension, can be identified using cell
lines from general pedigrees selected without any knowledge of the
blood pressure status of the donors. This strategy represents an
approach to rapidly and inexpensively mapping loci related to
common, complex disorders, using phenotypes that are stable in
immortalized lymphoblasts together with existing reference pedigree
cell lines and genotype databases.
