- Email: [email protected]
Panel discussion: Purification, structure, cDNA probes
PANEL DISCUSSIONz PURIFICATION, !SIWJC.TURE,cDNA PROBES
Chairperson:
Panel:
Hilton A. Salhanick Center for Population Studies Harvard Uedical School 665 Huntington Avenue Boston, WA 02155, USA
Evan R. Simpson University of Texas Southwestern Medical School 5325 Harry Hines Boulevard Dallas, TX 75235, USA Yoshio Osawa Medical Foundation of Buffalo 73 High Street Buffalo, NY 14203. USA Larry E. Vickery University of California, Irvine Irvine, CA 92717, USA Peter F. Hall Prince of Wales Hospital High and Avoca Streets Randwick, NSW 2031, Australia
R. RABTER:
I
would ask that the panel members address several issues
raised in their presentations. suggested the sion on
biochemical
Perhaps one for them. species?
presence of
of the
Specifically, previous
aromatase isozymes.
purification
showed
no
This morning's discusevidence
for isozymes.
panel members could review the biological evidence
How different are the aromatases
studied in
various animal
For instance, Dr. Gloria Callard finds that the Km for aroma-
tase in goldfish brain is about 2 nmol, 15-30 nmol.
Would
whereas, in
the human,
it is
one of the panel members also address the issue of
specificity of the P-450
reductases?
Does
cause any specificity in the aromatase system?
STEROIDS
reports have
50 / l-3 1987
the
reductase component
Perhaps Dr. Osawa could
308
Salhanick et ai.
discuss the type I and type II aromatases sgo and
comment on
testosterone.
that he
their relative specificity for androstenedione and
In addition, could a
panel member
comments on the P-450 superfamily of genes? P-45&
fit into the
lating P-450s
proposed same years
scheme,
such as
and,
For instance, how do liver
specifically, the steroid-hydroxy-
those mediating
450s have greater homology
make some background
6p-hydroxylation? Do these P-
with placental
aromatase than
some of the
other p-450s in liver? In.VICIIKPY:
As
I said
in my
talk, we
see no evidence for multiple
forms.
Terminal sequences described by our group and by other investi-
g&OX-S
suggest
only
a
single
except for partial truncation. with all
intermediates and
species
in our purified preparation,
The preparation we
all substrates.
have seems
to work
I see no reason to invoke
isozymes at this time. UN~XIPPIFIED PARYICIPZWC:
May I ask a follow-up question?
Was anyone
isolated aromatases from tissues other than the placenta; and more specifically, has anyone looked at Northern blots of
the aramatase clones
in tumors, to see if the m.RHhs might be different? C
uBt?Dl?zsSBz
We
have
used our cDNA probe against human placental
aromatase to test a number of different tissues losa cells,
rat granulosa
Simpson showed, there are encode for
this protein
cells, and
no indication
three
placenta.
human ovary and granulosa cells, and We have
human placenta
approximately in the
including human granu-
in rat
itself.
species
of
As Dr.
mRNA that
We see the same species in granulosa cells
as well.
to date that there are aromatase mRNA-size dif-
STEROlDS 5011-3 1987
PANEL DISCUSSiON
ferences in different tissues.
309
Presumably, there are haloes
speciesof this protein. We believe that there is just one form. R.
EMMTER:
El.-cX:
What is the biologicalevidencefor isozymes? I don't think that there is anyone on this panel who
would propose that there is biologicalevidence for isozymes. Y, asnWA: What I describedas isozymesare isofunctional enzymes that are recognizeddifferentlyby our monoclonaland polyclonalantibodies. The epitope capable of suppressingenzyme activityby antibodybinding must be near or at the active site of the enzyme. The antibodiesare raised against the cytochrome P-450 portion.
Aromatase is a complex
enyzme system, and the cytochromeP-450 portion is only a part of it. The only isozymesthat we have found so far by this approach are isozymes among differentspecies. Initially,I expectedthat point mutations would have occurredduring the process of evolutionand that the amino acid sequencesw0tda differ among species. Yet, as far as the active site of aromataseis concerned, I thought that the amino acid sequencesat that region would be more closely conserved. I didn't expect that our monoclonal antibody would differentiate among the aromatase enzyme% present in differentspecies through differential suppressionof enzyme activity. However, the fact is that there is immunochemicalevidence for differences among species,at or near the active site of aromatasecytochromeP-450. Several years ago, we
reportedmultiple forms of arcmatasefrom
human placenta. We called these activitiesP2 and P3. We consistently observed,as for many P-450s studied,that if we solubilize and separ-
STEROIDS 50 / 1-3 1987
310
Salhanick et al.
ate the cytochrome P-450 fraction from the reductase fraction, there is no evidence for biochemical separation of the P-450s. solubilize
them
so
that
they
and P3 aromatase. the
P2
as I
When we
cannot
make
estriol,
a difference,
different
reductase.
oxido-reductases besides
One interconverts androgenic,
steroids; one
these data.
We see
the NADPH cytochrome P-450 17-keto-,
and 17P-hydroxy-
interconverts estrone and estradiol; and the last, which
is present in different animal species, estriol but
in that
while P3 will make estriol.
There are some complications in interpreting three
apply immunoaffin-
described, we get a single P-450 from both P2
In the active form, there is
aromatase
if we
retain the aromatase activity, we can
consistently separate the different forms. ity chromatography
However,
converts 16a-hydroxyestrone to
not estriol to 16a-hydroxyestrone. These can be separated
by the column chromatography used for separation of the multiple forms. One explanation
is that
the solubilised
active aromatase
has a good
I.l(+hydroxyestrogendehydrogenaae, but no 16a-hydroxyestrone reductase; therefore, there is no estriol formation.
16a-Hydroxytestosterone is a
very poor substrate to be directly converted to estriol. These species of
observations
do
cytochrome P-450.
not
address
the
question
We simply don't know.
of different
The P3 aromatase
carries an activity that reduces 16a-hydroxyestrone to estriol. oxido-reductase has
not been
fully characterized. The complex struc-
ture of lipid plus aromatase plus other enzymes bound
in
nature.
I
This
appears to
be tightly
could conceive that, biologically, the site to
which these oxido-reductases are complexed could make a difference.
STEROIDS
50 / l-3 1987
PANEL DISCUSSION
311
Another question relatesto the nature of the reductases. The liver microsomal NADPH cytochrome P-450 reductase frcnnother species efficientlycouples to purifiedaromataseP-450. However, ismunochemical suppression studies suggest speciesdifferences,particularlyin horse placentas. The efficiencyof couplinqof the solubilizedcytochrome P-450 of the P2 fractionalso shows a difference. The reductase that we isolate from human placenta couples best.
If we couple with
reductasefrom other sources such as porcine,rat, bovine, and rabbit liver, we see only S-20% of aromataseactivityeven if we increasethe amount of reductase. On that issue, Casper has shown that there is only one
E.SlMpNN:
reductasegene. This presumablycodes for the same reductaseno matter what organ it is in and this reductasepresumablycouples with every other cytochromeP-450 in the body. It is a
little hard to visualize
why placental reductasewould couple better than reductasefrom liver. What might be importantis the species differencerather than the organ difference. H. SAIJiMICK: Would you assume that the mitochrondrialreductasesare the same as the microsomalenzymes? E.SIWpSOW: No, these are different. ~~P~~
Could Dr. Hall comment on the ability of
lip-hydroxylase to 19-hydroxylatesteroid substrateand the possibility of contamination betweenmitochondrial Up-hydroxylase and microsomal aromatase?
STEROIDS
50 I l-3 1987
312
Salhanick
P. Hw:
et al.
There is no possibility of serious contamination between the
mitochondrial lip-hydroxylase and the not usually
expressed in
the same
bovine adrenal cortical mitochondria molecular model, from 18.
microsomal aromatase.
tissues.
They are
The lip-hydroxylase from
will also
19-hydroxylate.
On a
the 19-methyl is the same distance from 119 as lip is
The possibility would be that the substrate can fit
when you
get it out of the microsomal membrane, and perhaps it is a more permissive environment. site, and
The substrate might fit in two ways
I suppose
hydroxylation, it occur there.
That
that once
you have
is conceivable
into the active
started the process with 19-
that the
second hydroxylation would
would be almost routine for a P-450 that can start
the mechanism off. UNILZNTIFIED PARTICIPANT:
Is it possible that a
separate 19-hydroxyl-
ase enzyme exists? E.SIHPSON:
As you know, there is a very active 19-hydroxylase in the so I
adrenal of some species -- the gerbil, for example -it is
think that
quite a likely possibility that there is a 19-hydroxylase, which
is an independent entity from the aromatase as
such, in
some species.
It might be the second member of the cytochrome P-450 gene family XIX. To try to answer the question of the biosyn-
UNILZNTIFIED PARTICIPANT: thesis of 19-nor steroids, show that
presented at
this meeting to
porcine granulosa cells convert both androstenedione and 19-
hydroxyandrostenedione to aromatase
evidence was
inhibitors,
19-norandrostenedione. 4_hydroxyandrostenedione,
We
find
that the
aminoglutethimide
phosphate, and ketoconazole, all inhibit the conversion of both precur-
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
sors to
313
19-norandrostenedione.We suggest that the formationof 19-
norsteroidsis not a cytochromeP-450-mediatedevent, even based on the evidencewe have. Whether this reaction is catalyzedby the aromatase enzyme, I can't say at the moment. L. VEKERY:
Some of these questionsmay be answered,in part, when the
Dallas group is able to express the recombinantprotein and then assay the activitiesof the recombinantproteinsproduced from a single gene. B.SIM?SM:
When we get a full-lengthclone, that will become a possi-
bility. p. SIm:
I have been fascinatedby the observationsof extraordin-
arily high levels of 19-norandrostenedione in ovarian follicularfluid. It seems to me that if there were a mechanismwhereby the aromatization process could be aborted at that step, this might be a very important controlpoint in terms of the amount of estrogenssecreted,or of a compoundwhich may have totally different properties that we don't recognizeat the present time. This, then, raises the questionwhether anyone can propose a mechanismthat would abort the aromatase so that 19-norsteroidis secreted. Y. OSAWA:
We have shown the enzyme system which we call non-aromatiz-
ing 19-hydroxylasein the dog and sheep adrenal.
These tissuesmay
have high androstenedione 19-hydroxylase activityand showed an apparent isotope effect of about 11.7, which is obviouslydifferentfrom that of the aromatase. We have not characterizedthe enzyme, but it proceeds to form the 19-aldehydeand also 19-norandrogen. It results in very little estrogen synthesis.
STEROIDS
50 I l-3 1987
I don't really understandthe
314
Salhanicket a/.
nature of this enzyme; it could be the same P-450 as the aromatase, but with
something
second stage. have shown
else
regulating
diverting
or
the process after the
Alternatively, it may be a totally different enzyme.
We
that it is a cytochrome P-450-dependent process, but beyond
that we don't know much about it. F._LrW:
I believe it of interest to show how powerful
antibody directed
against aromatase
localizing and understanding performed
the
can be,
synthesis
immunocytochemistry using
Dr.
particularly in terms of of
We have
In the upper
left (Fig-
the syncytiotrophoblasts are clearly marked, whereas the cyto-
trophoblasts are clear and the aromatase only
in the
nuclei
show
serum which
no
has apparently
our own
Finally, in Figure 3, one can see
the syncytiotrophoblasts, aromatase is
expect it, not in the nucleus but in shows an
polyclonal anti-
the same distribution, being found only in
the syncytiotrophoblasts (Figure 2).
The insert
There is
activity.
syncytiotrophoblasts. That can be seen by com-
paring it with estradiol dehydrogenase using
that in
aromatase.
Simpson and Dr. Mendelson's
antiserum to study human placental aromatase. ure l),
a tool the
area of
the rough
found where one might endoplasmic‘reticulum.
golgi with no evidence of immunopositive Thus, aromatase -in vitro
material being processed within it.
can be
seen to be limited to the microsomes. uNIDEt?rIFIEDPARTICIPANT: mediate production. first
studied,
the
I would like to bring up the topic of inter-
Back in the 1950s and biosynthetic
hydroxylation for two reasons.
1960s when
aromatases were
activity was thought to involve 19-
First, the 19-hydroxy and 19-oxo deriv-
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
315
1. Photomicrographs of human first trimester placenta Wostained for arcmatase cytochrome P-450. (a) Iranunostaining in the syncytiotrophoblast cytoplasm while the nuclei are consistently unstained. (b) Consecutive section to (a) showing complete abolition of irnrmnostaining after incubation with antiserum preadsorbed with 500 pg purified cytochrome P-450,,,. (c) Section immunostained for aromatase cytochrome P-450 and counterstained with Mayer's hematoxylin. Cytotrophoblast cells are easily recognized (arrows) and appear free of staining. (d,e) The inununoperoxidase has been replaced by a goldsilver intensification technique. Ivununoreactiveproduct appearing as a dense black precipitate is seen in the syncytiotrophoblast cells only. The unstained nuclei appear as small white dots. Orisinal magnifications: a,b,c,e, x100_ a, x20. Reprinted with permission of the authors and publisher (J CLIN ENDOCRINOL METAB 65:757, 1987). FIaJRE
STEROIDS
50 / l-3 1987
316
Salhanick et a/.
PIGOREZ2. Photomicrographs of human first trimester placenta immunostaining for E2DH. (a) General view of the chorionic villi, showing intense immunostaining of the syncytiotrophoblast layer only. Note the homogeneous and dense distribution of the peroxidase reaction product that, when seen in the cytoplasm in these thick sections, could account for apparent immunostaining over the nuclei. Some unstained nuclei (b) Higher magnification, emphasizing the appear as white dots. absence of staining of the cytotrophoblast cells (arrows). Original Reprinted with permission of the magnifications: a, x20; b, x100. authors and publisher (J CLIN ENDOCRINOL METAB 65:757, 1987).
STEROIDS
50 / 1-3 1987
PANEL DISCUSSION
317
Electron micrographs of human first trimesterplacenta EMJRB 3. irmrunostained for aromatasecytochromeP-450. (a) General appearanceof a syncytial cell (St). Peroxidasereactionproduct is concentratedin the cytoplasmand covers the endoplasmicreticulum(arrows). Note the absence of stainingof the microvilli(mv) and adjacentcytotropboblast cells (ct). fb) Higher magnificationof the area outlined in a, showing the absence of stainingof the Golgi apParatusand secretorygranules. Bar scales f 1 pm. Reprinted with permission of the authors and publisher (J CLIN VINYL HaTAR 65:757, 1987).
STEROIDS 50 I I-3 1987
318
Salhanick
atives
were
et al.
detected in the medium in relatively large quantities early
and appeared sequentially. Now, when
substrates.
Second,
we examined
they
were
data from
efficiently
the purified enzyme (I
think I first noticed this in Dr. Peter Hall's publication then in
Dr. Dwain
Hagerman's paper
and Dr.
used as
in BBRC and
Osawa's studies using 2-
dimensional TLC), it seemed to me that there was very little intermediate produced.
Could the speakers comment on that?
L. VICKERY:
There is a possibility that this may be due to the rate of
delivery of
reducing
equivalents.
When
the
delivery
of reducing
equivalent to the enzyme is slow, there is a greater probability of the intermediate products dissociating or trations of the substrate.
being displaced
by high concen-
I think Dr. Peter Hall has carried out some
very elegant experiments with the 17-hydroxylase, showing that have release
of 17-hydroxy intermediates from the hydroxylase lyase at
limiting reductase concentrations.
Isn't that correct?
p. HALL:
It is certainly true that we don't think of
P-450 as
rate-limiting in
tions.
limiting.
another cycle
the reduction of
the ordinary liver-drug hydroxylation reac-
When the enzyme has more than
it requires
you can
one hydroxylation
to carry out,
of reduction and then reductase does become
If you start, for example, with the C-21 side-chain cleavage
enzyme and incubate with progesterone, you can measure both 17a-hydroxylation and the lyase reaction which cleaves off the acetate. Vmax values
for that last step are always much lower than if you start
with 17a-hydroxyprogesterone as the substrate. of reduction
Now, the
may be
I think
that the rate
a factor in allowing the release of intermediates
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
319
which may not occur when the reductase activity is adjusted in the microsome-in vivo. We don't really know very much about that yet. Dr. Leo Samuelsperformeda series of
elegant experiments with microsomes
from testis showing that when the 17a-hydroxyprogesterone is added to the water phase it does not compete well
with the 17-hydroxyprogester-
one generated on the surface of the enzyme.
Once you get it out of the
microsomal membrane, all sorts
of intermediates would be
of spillage
possible.
L.vIclcKRY: I think Dr. Bellino suggested some time ago that reductase can be partially rate-limiting in the microsomal system tion.
In fact,
we have
reductase, at least
in
almost
rate
double
the
found that
the of
by supplementing microsomes with
detergent-reconstituted
and adding
tase will cause the rate to go up at least 50%. reductase may
system,
we can
aromatization without adding more P-450.
Simply dispersing the microsomes in detergent
that the
for aromatiza-
be partially
extra reduc-
There is some evidence
rate-limiting -in
situ, and this
could lead to more spillover of the intermediates. P. SIIYERI:
I
would like to cosunentthat we showed clearly, in 1974,
that the ratio of metabolites that one observes is totally dependent on the substrate
concentration at the start.
It was first suggested that
the rate-limiting step was, in fact, 19-hydroxylation, because very low substrate levels period of time.
were used and it was totally consumed in a very short We showed
that, with
very high
fact, the third hydroxylation is rate-limiting. what the rates are -in vivo, the enzyme
STEROIDS
50 / l-3 1987
is far
substrate levels, in If you try to estimate
from saturation
in the
320
Salhanick et a/.
placenta.
One would expect that the reductase may or may not be rate-
limiting, but clearly you don't see a lot or 19"norandrostenedione in pregnancy.
of ~9-hydro~androstenedione So
it is
running very effi-
ciently.
P. HALL:
Dr. Cisawa,I would like to reopen the "19-nor" question.
you able
to say anything about the way in which the aldehyde moiety is
lost from the f9-formyl or the 19-aldehyde in hydroxylase?
the case
of the adrenal
Does it come off as formic acid or COz?
Y. OSAWA:
Your
mechanism.
I am not prepared to answer that question
trying to
Are
question relates
to the non-aromatizing 19-desmolase as yet.
We are
meke an androgen labeled with I*C at the 19 position so that
we can identify the fate of that 19-carbon for sure. on tritium-labeled
substrates, I
would guess
stead of formaldehyde is lost in the case
From
our studies
that carbon dioxide in-
of non-aromatizing 19-desmo-
lation. D. PUETT:
I
wanted to ask about Dr. Hall's Km values, which seemed a
bit high. P. HALL:
These are all
aqueous phase
in
Vmax over
liposomes with
and phosphatidylcholine. between
which the
enzyme is
with no special detergent present.
fold lower and the enzyme
values in
preparations
3 times
higher if
present in an
The Km values are 5you reconstitute the
an equal mixture of phosphatidylethanolamine Based on this,
that
we
have
I think
that the differences
seen today may be related to the
detergent that is still present after purification or that is
added in
the reconstitution procedure.
STEROIDS 50 / 1-3 1987
PANEL DISCUSSION
H.
Regarding
BRODIB:
the
question
Simpson or Dr. Hall might speculate tions and
what they
expect to
321
of regulation, I wonder if Dr.
about post-translational modifica-
find with respect to the regulation of
aromatase? EE.SIHExm:
Since
this is,
of course,
an enzyme
of the endoplasmic
reticulum, one presumably would not expect to find any sequence modification in terms of loss of a precursor in the the enzyme
into the
endoplasmic reticulum.
process of
insertion of
From that point of view,
the product of _in vitro translation appears to be identical that found
in the
cell at
cleavage of a leader protein of
any given
moment.
sequence, which
the endoplasmic
is what
reticulum.
cell.
can In
also
occur
terms
glycosylation, I
of
if
There appears to be no you would
expect for a
Of course, the standard post-
translational modification of these enzymes is This
in size to
the insertion
of heme.
you express the cDNA in a non-steroidogenic
other
guess that
post-translational modifications this issue
has not
such as
been addressed, so I
have no knowledge of that. P. EALL:
It would have to be a guess,
but we
couldn't find
any evi-
dence of the aromatase being a glycoprotein. B
PARTICIPANT:
back to the old days. with placental
Another
All the
microsomes, but
question can be raised that goes
discussants this it has
morning have started
been reported
and observed in
many different laboratories that half of the total activity in placenta comes down
with the
mitochondrial fraction.
STEROIDS
50 / l-3 1987
Is that just due to con-
322
Salhanick et al.
tamination of the lower fractions with endoplasmic reticulum or are you confident that there is not a mitochondrial enzyme in placenta as well? I can comment on that.
L. VICKERY:
I don't know that we can rule out
other locations of the enzyme, but it is difficult to remove microsomes from nuclear debris and from mitochondrial pellets.
I know some of the
early isolation procedures actually threw away the microsomes the
debris
fractions
because
sedimented at low-g force. chondrial pellets of the activity is
so
much
and took
of the endoplasmic reticulum
If one takes the
debris pellets
and mito-
and rehomogenizes them and recentrifuges them, a lot then released
into the
so-called microsomal frac-
tion. P. HALL:
It certainly can be difficult to release endoplasmic reticu-
lum from the mitochondrial fraction. membrane shares
direct continuity
In fact,
the outer mitochondrial
with the endoplasmic reticulum.
least in our hands, I can say that less than 10% of
At
the total activity
of aromatase could be found in the mitochondrial fraction. LlNIDFN!IFIEDPARTICIPANT:
This
isn't a
the distribution of the aromatase. that it
is primarily
found in
In human placenta, it
the microsomes.
cently been examining sheep placenta. specific activity
of aromatase
question, it is a comment on
We find
in homogenate
However, we have re-
that if
we measure the
compared to that in the
classical microsomal fraction, the specific activity is only one-fourth that in the microsomes.
would appear
in the homogenate
One could predict from this
that there is aromatase activity in other fractions. When we looked at the so-called
heavy-light mitochondria-peroxisomal fraction, there was
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
a considerableamount of aromataseactivity there.
323
It could well be
that, in other tissues, there ie aromatasedistributedthroughmany membrane fractions. I think it will be staining studies to
interesting when people do
see if other fractions,specificallyin other
tissues like sheep placenta, and not just in human placenta,contain aromatase. It is still an open question,I think. F.NAFTOLIN: On careful examinationof electronmicrographsof inxnunohistochemicallystainedmaterial,the outer mitochondrialmembrane does stain, whereas the mitochondriathemselvesdo not -- neither the cristae nor any of the spaces within the mitochondria. The endoplasmic reticulumis really packed with aromatase-staining material. If aromatase is a mitochondrialenzyme: (a) it is evanescent,and be present in a relativelysmall amount.
STEROIDS 50 / f-3 1987
(b) it must
Chairperson:
Panel:
Hilton A. Salhanick Center for Population Studies Harvard Uedical School 665 Huntington Avenue Boston, WA 02155, USA
Evan R. Simpson University of Texas Southwestern Medical School 5325 Harry Hines Boulevard Dallas, TX 75235, USA Yoshio Osawa Medical Foundation of Buffalo 73 High Street Buffalo, NY 14203. USA Larry E. Vickery University of California, Irvine Irvine, CA 92717, USA Peter F. Hall Prince of Wales Hospital High and Avoca Streets Randwick, NSW 2031, Australia
R. RABTER:
I
would ask that the panel members address several issues
raised in their presentations. suggested the sion on
biochemical
Perhaps one for them. species?
presence of
of the
Specifically, previous
aromatase isozymes.
purification
showed
no
This morning's discusevidence
for isozymes.
panel members could review the biological evidence
How different are the aromatases
studied in
various animal
For instance, Dr. Gloria Callard finds that the Km for aroma-
tase in goldfish brain is about 2 nmol, 15-30 nmol.
Would
whereas, in
the human,
it is
one of the panel members also address the issue of
specificity of the P-450
reductases?
Does
cause any specificity in the aromatase system?
STEROIDS
reports have
50 / l-3 1987
the
reductase component
Perhaps Dr. Osawa could
308
Salhanick et ai.
discuss the type I and type II aromatases sgo and
comment on
testosterone.
that he
their relative specificity for androstenedione and
In addition, could a
panel member
comments on the P-450 superfamily of genes? P-45&
fit into the
lating P-450s
proposed same years
scheme,
such as
and,
For instance, how do liver
specifically, the steroid-hydroxy-
those mediating
450s have greater homology
make some background
6p-hydroxylation? Do these P-
with placental
aromatase than
some of the
other p-450s in liver? In.VICIIKPY:
As
I said
in my
talk, we
see no evidence for multiple
forms.
Terminal sequences described by our group and by other investi-
g&OX-S
suggest
only
a
single
except for partial truncation. with all
intermediates and
species
in our purified preparation,
The preparation we
all substrates.
have seems
to work
I see no reason to invoke
isozymes at this time. UN~XIPPIFIED PARYICIPZWC:
May I ask a follow-up question?
Was anyone
isolated aromatases from tissues other than the placenta; and more specifically, has anyone looked at Northern blots of
the aramatase clones
in tumors, to see if the m.RHhs might be different? C
uBt?Dl?zsSBz
We
have
used our cDNA probe against human placental
aromatase to test a number of different tissues losa cells,
rat granulosa
Simpson showed, there are encode for
this protein
cells, and
no indication
three
placenta.
human ovary and granulosa cells, and We have
human placenta
approximately in the
including human granu-
in rat
itself.
species
of
As Dr.
mRNA that
We see the same species in granulosa cells
as well.
to date that there are aromatase mRNA-size dif-
STEROlDS 5011-3 1987
PANEL DISCUSSiON
ferences in different tissues.
309
Presumably, there are haloes
speciesof this protein. We believe that there is just one form. R.
EMMTER:
El.-cX:
What is the biologicalevidencefor isozymes? I don't think that there is anyone on this panel who
would propose that there is biologicalevidence for isozymes. Y, asnWA: What I describedas isozymesare isofunctional enzymes that are recognizeddifferentlyby our monoclonaland polyclonalantibodies. The epitope capable of suppressingenzyme activityby antibodybinding must be near or at the active site of the enzyme. The antibodiesare raised against the cytochrome P-450 portion.
Aromatase is a complex
enyzme system, and the cytochromeP-450 portion is only a part of it. The only isozymesthat we have found so far by this approach are isozymes among differentspecies. Initially,I expectedthat point mutations would have occurredduring the process of evolutionand that the amino acid sequencesw0tda differ among species. Yet, as far as the active site of aromataseis concerned, I thought that the amino acid sequencesat that region would be more closely conserved. I didn't expect that our monoclonal antibody would differentiate among the aromatase enzyme% present in differentspecies through differential suppressionof enzyme activity. However, the fact is that there is immunochemicalevidence for differences among species,at or near the active site of aromatasecytochromeP-450. Several years ago, we
reportedmultiple forms of arcmatasefrom
human placenta. We called these activitiesP2 and P3. We consistently observed,as for many P-450s studied,that if we solubilize and separ-
STEROIDS 50 / 1-3 1987
310
Salhanick et al.
ate the cytochrome P-450 fraction from the reductase fraction, there is no evidence for biochemical separation of the P-450s. solubilize
them
so
that
they
and P3 aromatase. the
P2
as I
When we
cannot
make
estriol,
a difference,
different
reductase.
oxido-reductases besides
One interconverts androgenic,
steroids; one
these data.
We see
the NADPH cytochrome P-450 17-keto-,
and 17P-hydroxy-
interconverts estrone and estradiol; and the last, which
is present in different animal species, estriol but
in that
while P3 will make estriol.
There are some complications in interpreting three
apply immunoaffin-
described, we get a single P-450 from both P2
In the active form, there is
aromatase
if we
retain the aromatase activity, we can
consistently separate the different forms. ity chromatography
However,
converts 16a-hydroxyestrone to
not estriol to 16a-hydroxyestrone. These can be separated
by the column chromatography used for separation of the multiple forms. One explanation
is that
the solubilised
active aromatase
has a good
I.l(+hydroxyestrogendehydrogenaae, but no 16a-hydroxyestrone reductase; therefore, there is no estriol formation.
16a-Hydroxytestosterone is a
very poor substrate to be directly converted to estriol. These species of
observations
do
cytochrome P-450.
not
address
the
question
We simply don't know.
of different
The P3 aromatase
carries an activity that reduces 16a-hydroxyestrone to estriol. oxido-reductase has
not been
fully characterized. The complex struc-
ture of lipid plus aromatase plus other enzymes bound
in
nature.
I
This
appears to
be tightly
could conceive that, biologically, the site to
which these oxido-reductases are complexed could make a difference.
STEROIDS
50 / l-3 1987
PANEL DISCUSSION
311
Another question relatesto the nature of the reductases. The liver microsomal NADPH cytochrome P-450 reductase frcnnother species efficientlycouples to purifiedaromataseP-450. However, ismunochemical suppression studies suggest speciesdifferences,particularlyin horse placentas. The efficiencyof couplinqof the solubilizedcytochrome P-450 of the P2 fractionalso shows a difference. The reductase that we isolate from human placenta couples best.
If we couple with
reductasefrom other sources such as porcine,rat, bovine, and rabbit liver, we see only S-20% of aromataseactivityeven if we increasethe amount of reductase. On that issue, Casper has shown that there is only one
E.SlMpNN:
reductasegene. This presumablycodes for the same reductaseno matter what organ it is in and this reductasepresumablycouples with every other cytochromeP-450 in the body. It is a
little hard to visualize
why placental reductasewould couple better than reductasefrom liver. What might be importantis the species differencerather than the organ difference. H. SAIJiMICK: Would you assume that the mitochrondrialreductasesare the same as the microsomalenzymes? E.SIWpSOW: No, these are different. ~~P~~
Could Dr. Hall comment on the ability of
lip-hydroxylase to 19-hydroxylatesteroid substrateand the possibility of contamination betweenmitochondrial Up-hydroxylase and microsomal aromatase?
STEROIDS
50 I l-3 1987
312
Salhanick
P. Hw:
et al.
There is no possibility of serious contamination between the
mitochondrial lip-hydroxylase and the not usually
expressed in
the same
bovine adrenal cortical mitochondria molecular model, from 18.
microsomal aromatase.
tissues.
They are
The lip-hydroxylase from
will also
19-hydroxylate.
On a
the 19-methyl is the same distance from 119 as lip is
The possibility would be that the substrate can fit
when you
get it out of the microsomal membrane, and perhaps it is a more permissive environment. site, and
The substrate might fit in two ways
I suppose
hydroxylation, it occur there.
That
that once
you have
is conceivable
into the active
started the process with 19-
that the
second hydroxylation would
would be almost routine for a P-450 that can start
the mechanism off. UNILZNTIFIED PARTICIPANT:
Is it possible that a
separate 19-hydroxyl-
ase enzyme exists? E.SIHPSON:
As you know, there is a very active 19-hydroxylase in the so I
adrenal of some species -- the gerbil, for example -it is
think that
quite a likely possibility that there is a 19-hydroxylase, which
is an independent entity from the aromatase as
such, in
some species.
It might be the second member of the cytochrome P-450 gene family XIX. To try to answer the question of the biosyn-
UNILZNTIFIED PARTICIPANT: thesis of 19-nor steroids, show that
presented at
this meeting to
porcine granulosa cells convert both androstenedione and 19-
hydroxyandrostenedione to aromatase
evidence was
inhibitors,
19-norandrostenedione. 4_hydroxyandrostenedione,
We
find
that the
aminoglutethimide
phosphate, and ketoconazole, all inhibit the conversion of both precur-
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
sors to
313
19-norandrostenedione.We suggest that the formationof 19-
norsteroidsis not a cytochromeP-450-mediatedevent, even based on the evidencewe have. Whether this reaction is catalyzedby the aromatase enzyme, I can't say at the moment. L. VEKERY:
Some of these questionsmay be answered,in part, when the
Dallas group is able to express the recombinantprotein and then assay the activitiesof the recombinantproteinsproduced from a single gene. B.SIM?SM:
When we get a full-lengthclone, that will become a possi-
bility. p. SIm:
I have been fascinatedby the observationsof extraordin-
arily high levels of 19-norandrostenedione in ovarian follicularfluid. It seems to me that if there were a mechanismwhereby the aromatization process could be aborted at that step, this might be a very important controlpoint in terms of the amount of estrogenssecreted,or of a compoundwhich may have totally different properties that we don't recognizeat the present time. This, then, raises the questionwhether anyone can propose a mechanismthat would abort the aromatase so that 19-norsteroidis secreted. Y. OSAWA:
We have shown the enzyme system which we call non-aromatiz-
ing 19-hydroxylasein the dog and sheep adrenal.
These tissuesmay
have high androstenedione 19-hydroxylase activityand showed an apparent isotope effect of about 11.7, which is obviouslydifferentfrom that of the aromatase. We have not characterizedthe enzyme, but it proceeds to form the 19-aldehydeand also 19-norandrogen. It results in very little estrogen synthesis.
STEROIDS
50 I l-3 1987
I don't really understandthe
314
Salhanicket a/.
nature of this enzyme; it could be the same P-450 as the aromatase, but with
something
second stage. have shown
else
regulating
diverting
or
the process after the
Alternatively, it may be a totally different enzyme.
We
that it is a cytochrome P-450-dependent process, but beyond
that we don't know much about it. F._LrW:
I believe it of interest to show how powerful
antibody directed
against aromatase
localizing and understanding performed
the
can be,
synthesis
immunocytochemistry using
Dr.
particularly in terms of of
We have
In the upper
left (Fig-
the syncytiotrophoblasts are clearly marked, whereas the cyto-
trophoblasts are clear and the aromatase only
in the
nuclei
show
serum which
no
has apparently
our own
Finally, in Figure 3, one can see
the syncytiotrophoblasts, aromatase is
expect it, not in the nucleus but in shows an
polyclonal anti-
the same distribution, being found only in
the syncytiotrophoblasts (Figure 2).
The insert
There is
activity.
syncytiotrophoblasts. That can be seen by com-
paring it with estradiol dehydrogenase using
that in
aromatase.
Simpson and Dr. Mendelson's
antiserum to study human placental aromatase. ure l),
a tool the
area of
the rough
found where one might endoplasmic‘reticulum.
golgi with no evidence of immunopositive Thus, aromatase -in vitro
material being processed within it.
can be
seen to be limited to the microsomes. uNIDEt?rIFIEDPARTICIPANT: mediate production. first
studied,
the
I would like to bring up the topic of inter-
Back in the 1950s and biosynthetic
hydroxylation for two reasons.
1960s when
aromatases were
activity was thought to involve 19-
First, the 19-hydroxy and 19-oxo deriv-
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
315
1. Photomicrographs of human first trimester placenta Wostained for arcmatase cytochrome P-450. (a) Iranunostaining in the syncytiotrophoblast cytoplasm while the nuclei are consistently unstained. (b) Consecutive section to (a) showing complete abolition of irnrmnostaining after incubation with antiserum preadsorbed with 500 pg purified cytochrome P-450,,,. (c) Section immunostained for aromatase cytochrome P-450 and counterstained with Mayer's hematoxylin. Cytotrophoblast cells are easily recognized (arrows) and appear free of staining. (d,e) The inununoperoxidase has been replaced by a goldsilver intensification technique. Ivununoreactiveproduct appearing as a dense black precipitate is seen in the syncytiotrophoblast cells only. The unstained nuclei appear as small white dots. Orisinal magnifications: a,b,c,e, x100_ a, x20. Reprinted with permission of the authors and publisher (J CLIN ENDOCRINOL METAB 65:757, 1987). FIaJRE
STEROIDS
50 / l-3 1987
316
Salhanick et a/.
PIGOREZ2. Photomicrographs of human first trimester placenta immunostaining for E2DH. (a) General view of the chorionic villi, showing intense immunostaining of the syncytiotrophoblast layer only. Note the homogeneous and dense distribution of the peroxidase reaction product that, when seen in the cytoplasm in these thick sections, could account for apparent immunostaining over the nuclei. Some unstained nuclei (b) Higher magnification, emphasizing the appear as white dots. absence of staining of the cytotrophoblast cells (arrows). Original Reprinted with permission of the magnifications: a, x20; b, x100. authors and publisher (J CLIN ENDOCRINOL METAB 65:757, 1987).
STEROIDS
50 / 1-3 1987
PANEL DISCUSSION
317
Electron micrographs of human first trimesterplacenta EMJRB 3. irmrunostained for aromatasecytochromeP-450. (a) General appearanceof a syncytial cell (St). Peroxidasereactionproduct is concentratedin the cytoplasmand covers the endoplasmicreticulum(arrows). Note the absence of stainingof the microvilli(mv) and adjacentcytotropboblast cells (ct). fb) Higher magnificationof the area outlined in a, showing the absence of stainingof the Golgi apParatusand secretorygranules. Bar scales f 1 pm. Reprinted with permission of the authors and publisher (J CLIN VINYL HaTAR 65:757, 1987).
STEROIDS 50 I I-3 1987
318
Salhanick
atives
were
et al.
detected in the medium in relatively large quantities early
and appeared sequentially. Now, when
substrates.
Second,
we examined
they
were
data from
efficiently
the purified enzyme (I
think I first noticed this in Dr. Peter Hall's publication then in
Dr. Dwain
Hagerman's paper
and Dr.
used as
in BBRC and
Osawa's studies using 2-
dimensional TLC), it seemed to me that there was very little intermediate produced.
Could the speakers comment on that?
L. VICKERY:
There is a possibility that this may be due to the rate of
delivery of
reducing
equivalents.
When
the
delivery
of reducing
equivalent to the enzyme is slow, there is a greater probability of the intermediate products dissociating or trations of the substrate.
being displaced
by high concen-
I think Dr. Peter Hall has carried out some
very elegant experiments with the 17-hydroxylase, showing that have release
of 17-hydroxy intermediates from the hydroxylase lyase at
limiting reductase concentrations.
Isn't that correct?
p. HALL:
It is certainly true that we don't think of
P-450 as
rate-limiting in
tions.
limiting.
another cycle
the reduction of
the ordinary liver-drug hydroxylation reac-
When the enzyme has more than
it requires
you can
one hydroxylation
to carry out,
of reduction and then reductase does become
If you start, for example, with the C-21 side-chain cleavage
enzyme and incubate with progesterone, you can measure both 17a-hydroxylation and the lyase reaction which cleaves off the acetate. Vmax values
for that last step are always much lower than if you start
with 17a-hydroxyprogesterone as the substrate. of reduction
Now, the
may be
I think
that the rate
a factor in allowing the release of intermediates
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
319
which may not occur when the reductase activity is adjusted in the microsome-in vivo. We don't really know very much about that yet. Dr. Leo Samuelsperformeda series of
elegant experiments with microsomes
from testis showing that when the 17a-hydroxyprogesterone is added to the water phase it does not compete well
with the 17-hydroxyprogester-
one generated on the surface of the enzyme.
Once you get it out of the
microsomal membrane, all sorts
of intermediates would be
of spillage
possible.
L.vIclcKRY: I think Dr. Bellino suggested some time ago that reductase can be partially rate-limiting in the microsomal system tion.
In fact,
we have
reductase, at least
in
almost
rate
double
the
found that
the of
by supplementing microsomes with
detergent-reconstituted
and adding
tase will cause the rate to go up at least 50%. reductase may
system,
we can
aromatization without adding more P-450.
Simply dispersing the microsomes in detergent
that the
for aromatiza-
be partially
extra reduc-
There is some evidence
rate-limiting -in
situ, and this
could lead to more spillover of the intermediates. P. SIIYERI:
I
would like to cosunentthat we showed clearly, in 1974,
that the ratio of metabolites that one observes is totally dependent on the substrate
concentration at the start.
It was first suggested that
the rate-limiting step was, in fact, 19-hydroxylation, because very low substrate levels period of time.
were used and it was totally consumed in a very short We showed
that, with
very high
fact, the third hydroxylation is rate-limiting. what the rates are -in vivo, the enzyme
STEROIDS
50 / l-3 1987
is far
substrate levels, in If you try to estimate
from saturation
in the
320
Salhanick et a/.
placenta.
One would expect that the reductase may or may not be rate-
limiting, but clearly you don't see a lot or 19"norandrostenedione in pregnancy.
of ~9-hydro~androstenedione So
it is
running very effi-
ciently.
P. HALL:
Dr. Cisawa,I would like to reopen the "19-nor" question.
you able
to say anything about the way in which the aldehyde moiety is
lost from the f9-formyl or the 19-aldehyde in hydroxylase?
the case
of the adrenal
Does it come off as formic acid or COz?
Y. OSAWA:
Your
mechanism.
I am not prepared to answer that question
trying to
Are
question relates
to the non-aromatizing 19-desmolase as yet.
We are
meke an androgen labeled with I*C at the 19 position so that
we can identify the fate of that 19-carbon for sure. on tritium-labeled
substrates, I
would guess
stead of formaldehyde is lost in the case
From
our studies
that carbon dioxide in-
of non-aromatizing 19-desmo-
lation. D. PUETT:
I
wanted to ask about Dr. Hall's Km values, which seemed a
bit high. P. HALL:
These are all
aqueous phase
in
Vmax over
liposomes with
and phosphatidylcholine. between
which the
enzyme is
with no special detergent present.
fold lower and the enzyme
values in
preparations
3 times
higher if
present in an
The Km values are 5you reconstitute the
an equal mixture of phosphatidylethanolamine Based on this,
that
we
have
I think
that the differences
seen today may be related to the
detergent that is still present after purification or that is
added in
the reconstitution procedure.
STEROIDS 50 / 1-3 1987
PANEL DISCUSSION
H.
Regarding
BRODIB:
the
question
Simpson or Dr. Hall might speculate tions and
what they
expect to
321
of regulation, I wonder if Dr.
about post-translational modifica-
find with respect to the regulation of
aromatase? EE.SIHExm:
Since
this is,
of course,
an enzyme
of the endoplasmic
reticulum, one presumably would not expect to find any sequence modification in terms of loss of a precursor in the the enzyme
into the
endoplasmic reticulum.
process of
insertion of
From that point of view,
the product of _in vitro translation appears to be identical that found
in the
cell at
cleavage of a leader protein of
any given
moment.
sequence, which
the endoplasmic
is what
reticulum.
cell.
can In
also
occur
terms
glycosylation, I
of
if
There appears to be no you would
expect for a
Of course, the standard post-
translational modification of these enzymes is This
in size to
the insertion
of heme.
you express the cDNA in a non-steroidogenic
other
guess that
post-translational modifications this issue
has not
such as
been addressed, so I
have no knowledge of that. P. EALL:
It would have to be a guess,
but we
couldn't find
any evi-
dence of the aromatase being a glycoprotein. B
PARTICIPANT:
back to the old days. with placental
Another
All the
microsomes, but
question can be raised that goes
discussants this it has
morning have started
been reported
and observed in
many different laboratories that half of the total activity in placenta comes down
with the
mitochondrial fraction.
STEROIDS
50 / l-3 1987
Is that just due to con-
322
Salhanick et al.
tamination of the lower fractions with endoplasmic reticulum or are you confident that there is not a mitochondrial enzyme in placenta as well? I can comment on that.
L. VICKERY:
I don't know that we can rule out
other locations of the enzyme, but it is difficult to remove microsomes from nuclear debris and from mitochondrial pellets.
I know some of the
early isolation procedures actually threw away the microsomes the
debris
fractions
because
sedimented at low-g force. chondrial pellets of the activity is
so
much
and took
of the endoplasmic reticulum
If one takes the
debris pellets
and mito-
and rehomogenizes them and recentrifuges them, a lot then released
into the
so-called microsomal frac-
tion. P. HALL:
It certainly can be difficult to release endoplasmic reticu-
lum from the mitochondrial fraction. membrane shares
direct continuity
In fact,
the outer mitochondrial
with the endoplasmic reticulum.
least in our hands, I can say that less than 10% of
At
the total activity
of aromatase could be found in the mitochondrial fraction. LlNIDFN!IFIEDPARTICIPANT:
This
isn't a
the distribution of the aromatase. that it
is primarily
found in
In human placenta, it
the microsomes.
cently been examining sheep placenta. specific activity
of aromatase
question, it is a comment on
We find
in homogenate
However, we have re-
that if
we measure the
compared to that in the
classical microsomal fraction, the specific activity is only one-fourth that in the microsomes.
would appear
in the homogenate
One could predict from this
that there is aromatase activity in other fractions. When we looked at the so-called
heavy-light mitochondria-peroxisomal fraction, there was
STEROIDS
50 / l-3
1987
PANEL DISCUSSION
a considerableamount of aromataseactivity there.
323
It could well be
that, in other tissues, there ie aromatasedistributedthroughmany membrane fractions. I think it will be staining studies to
interesting when people do
see if other fractions,specificallyin other
tissues like sheep placenta, and not just in human placenta,contain aromatase. It is still an open question,I think. F.NAFTOLIN: On careful examinationof electronmicrographsof inxnunohistochemicallystainedmaterial,the outer mitochondrialmembrane does stain, whereas the mitochondriathemselvesdo not -- neither the cristae nor any of the spaces within the mitochondria. The endoplasmic reticulumis really packed with aromatase-staining material. If aromatase is a mitochondrialenzyme: (a) it is evanescent,and be present in a relativelysmall amount.
STEROIDS 50 / f-3 1987
(b) it must