GLENN D. KUEHN
B.A. (Concordia College) 1964;
Ph.D. (Washington State) 1968;
Postdoctoral (UCLA)
1968;
Sabbatical
(University of Berne, Switzerland) 1978
gkuehn@nmsu.edu
(505)-646-1015
Dr. Kuehn has had an ongoing, active research program at New
Mexico State University since 1970. His research interests
have centered on several topics in polyamine metabolism and
roles in cellular homeostasis.
Synopsis:
Polyamine oxidase (PAO) catalyzes oxidative cleavage of
polyamines spermidine (spd) or spermine (spm) to produce
diaminopropane (dap), H2O2, and an aminoaldehyde derivative.
In plants, dap is the precursor for biosynthesis of
norspermidine (nspd) and norspermine (nspm) via the enzyme,
Schiff base reductase decarboxylase (SBRD). Recently, the
catabolism of spd and spm by PAO has been proposed by
several investigators to be a causative agent, through
product H2O2 and ensuing oxidative stress, which forces
animal cells into programmed cell death (apoptosis). The
gene for PAO from oat seedlings was recently cloned,
sequenced, and characterized in this laboratory. The
availability of this newly isolated gene offers unique
opportunities to gain genetic evidence for a potential
role(s) of PAO and polyamine-catabolism in apoptosis in a
plant model test system.
The hypothesis of this application is: (i) PAO has a
causative role in apoptosis in cells through H2O2 produced
by its oxidation of spd or spm, and (ii) the nspd and nspm
produced from dap serve as suppressors of apoptosis through
feedback inhibition of PAO and reduction in H2O2 synthesis.
The specific aims of this proposal are: (1) The PAO cDNA
gene sequence will be used to generate antisense PAO gene
constructs ligated to a copper-inducible promoter. These
constructs will be used to transform alfalfa plants with
Ti-plasmid methods to analyze the consequences of controlled
PAO-deficiency on apoptosis in plant tissues. (2) The cDNA
gene sequence for the enzyme, SBRD, which catalyzes nspd and
nspm biosynthesis from dap, will be used to generate
antisense SBRD gene constructs ligated to a copper-inducible
promoter. These constructs will be used to transform alfalfa
plants in order to analyze the consequences of uncoupling
generation of H2O2 by PAO from the biosynthesis of nspd and
nspm derived from dap by SBRD.
Aims (1) and (2) are direct tests of parts (i) and (ii) of
the hypothesis. (3) The PAO cDNA gene sequence from oat will
be used as a gene probe to attempt the isolation of the
human PAO gene from kidney and liver cDNA libraries. A
characterized human PAO gene will make possible the
development of a molecular biological approach to
investigate the role of PAO in generating H2O2 and its
alleged role to elicit animal apoptosis. (4) The cDNA gene
sequence of a signal peptide for the PAO gene will be
ligated to a gene coding for a green fluorescent protein (GFP).
The fusion protein produced from this construction will be
analyzed by fluorescent imaging techniques in tissues of
alfalfa and oat plants transformed with this construction in
order to identify the subcellular localization of PAO. In
situ labeling of PAO by immunogold antibody reagents and
electronmicroscopic analysis, will corroborate the
localization studies by the GFP fusion protein technique.
These results will aid in localizing the origin of events
that initiate PAO-dependent apoptosis.