Selecting
for tumor cells is very important for an assay like the MTT
assay, ATP assay, FDA assay, and caspase 3/7 assay, all of which use an
endpoint which can't discriminate between tumor cells and normal cells
(in contradistinction to the DISC assay, in which tumor-specific drug
effects can be distinguished in a mixed cell population). Serum
free medium and anchorage independent growing conditions will prevent
the _growth_ of normal cells but in most short term cell death assays
we are not measuring cell growth but rather cell survival. The
selective advantage of anchorage independence and serum free status is
much less in the case of short term cell survival than it is for actual
cell growth. One of my many pet peeves about this literature is
the cavalier use of the term "growth." Thus, it is important to
"purify" tumor cell clusters prior to plating them in short term
culture.
Here
are what our own data show (representative data shown for specimens
with an official histopathologic diagnosis of poory-differentiated
ovarian cancer):
Treatment
cohort (in ovarian cancer)
|
LC50
|
P2
(compared to "Relapsed < 6 months" cohort, below)
|
Previously Untreated (n=88)
|
1.53 ug/ml
|
=0.00015
|
Relapsed > 6 months post
platinum (n=45)
|
1.82 ug/ml
|
=0.0015
|
Relapsed < 6 months post
platinum (n=52)
|
2.43 ug/ml
|
(60% increase compared to
untreated)
|
Comments:
Methodology and patient survival correlations are presented in detail
elsewhere on this website). This isn't a scale model of
chemotherapy in the
patient. The LC50 value should not be used in the same fashion as an
anti-microbial "MIC" level, but the relative increase in effective
concentration is probably of clinical relevance (i.e. I think it would
take about a 60% increase in platinum dosage to achieve in the average
"platinum resistant" patient what could be achieved in the average
untreated patient).
Some selected technical details follow:
We've received a total of 946 specimens of ovarian cancer, fallopian
tube cancer, primary peritoneal papillary serous adenocarcinoma, and
papillary serous endometrial adenocarcinoma. All of these are now
considered to be essentially the same general "disease," from the
standpoint of biological behavior, response to treatment, and prognosis
in the Stage III/Stage IV setting. Most of these were simply
diagnosed as ovarian cancer.
Only
170 of these specimens had a post-culture to pre-culture
ratio of viable tumor cells which exceeded 1.01 (the definition of cell
"growth."). The median ratio was 0.85 and the mean ratio was
0.81. So you see, most of our specimens are not "growing."
Of our 946 specimens, most of the time the sources of cells was a solid
tumor biopsy or resection. In the case of the ascites fluid or
pleural fluid or pericardial fluid specimens (n=170), the median
post-culture/pre-culture viable tumor cell ratio was 1.0; however,
there was a distinct INCREASE (as opposed to simply 100% maintenance of
viability) in only 40 of 170 specimens.
In the
case of all 946 specimens, at the end of the culture
the median percent tumor cells (compared to normal cells) was 90% tumor
cells, compared to 10% normal cells. The corresponding means were
83% and 17% (meaning that some specimens had a whole lot of normal
cells at the end). In the case of the fluid specimens, the median
percent tumor cells at the end of culture was 90%, but the mean was
only 73%, meaning that some of the cultures had a very low percent
tumor cells (usually the "offending" normal cells in these latter cases
were mesothelial cells).
We
culture our cells in anchorage independent, polypropylene
microwells. I'm pretty sure that I was the
first investigator to report that polypropylene (as opposed to
polystyrene) provided anchorage independent growth conditions, in my
publications of the early 1980s. Maybe someone "scooped" me on
this; I'm not aware of it and, anyway, it's not all that big a
deal. We do a lot of work pre-culture to obtain relatively "pure"
populations of tumor cells. One of our bread and butter methods
was invented by my wife. It's something we call "quick
spins." Basically, mix up the cells in a centrifuge tube, turn on
the centrifuge (standard large benchtop Beckman TJ6 or Allegra6) and
barely let it get up to 1000-1500 RPM (depending on the specimen), then
immediately turn it off. The three dimensional cell clusters go
to the bottom; single cells, including dead cells and debris, stay in
the supernatant. Tumor cells are slightly more dense than are
mesothelial cells. With repeated 'quick spins' (sometimes up to
20 of them), you get a selective enrichment for tumor cells. We
monitor this process by making Cytospins along the way.
At the
end of the assay, we have many endpoints at our
disposal. In cases where there are many normal cells, the only
reliable endpoint is the DISC assay (which Robert Nagourney has
re-named the "Ex Vivo Apoptosis Assay" and which Andrew Bosanquet has
re-named the "TRAK" assay). We always run at least one and
usually two or even three additional endpoints. I prefer the MTT,
as it gives a very adequate signal in the typical ovarian specimen, and
it is more specific for tumor cells than other metabolic endpoints,
including the ATP. We also use resazurin and caspase 3/7 (using
the Promega Glo endpoint) for different purposes in different
situations, as well as the ATP (chiefly in situations where we have a
very pure population of tumor cells, but a very low cell yield).
I
don't know of a biological advantage in testing "pure"
tumor cells. Robert Hoffman makes a major point about maintaining
the native tumor architecture, including making sure that all the
normal cells are present. So he claims it's a biologically better
model to have all the normal cells present. But his published
correlations are just as good or bad as everyone else's (patients
treated with assay-active drugs much more likely to respond and live
longer). The only advantage in selectively culturing tumor cells
is if you use an endpoint which can't discriminate between normal cells
and tumor cells.
Everyone
in this field likes to claim that his/her method is
the best. I'm pretty sure that I'm about the only one working in
this field (well, maybe Larssen and Nygren in Uppsala; Kaspers and
Peters in Amsterdam also) who is happy to admit that all of the cell
death endpoints can be made to give equally valid information, if they
are done properly. The choice of which to use depends mostly an a
variety of technical factors relating to type of specimen.
I'm
also unaware that there is any advantage at all in using
serum free culture conditions, beyond providing selectivity for tumor
cell growth (true growth, as opposed to merely survival in short term
culture, where the selectiveness of serum-free culture is of much
lesser magnitude). One could make the case that having serum in
the medium makes it much more "physiological," as many drugs bind to
albumin and other proteins "naturally" present in the bloodstream (and
often in malignant ascites fluid). Without serum, there is less
binding, and lower in vitro concentrations of some drugs need to be
used to provide a proper "scatter" of results. But this is just a
matter of calibrating drug concentrations for the given assay
conditions. Everyone does it (calibrates his/her own assay for
differing conditions of culture).
In
short, I think that we (who work in this field) are all
good guys and that none of us are selective technical geniuses.
The toweringly impressive achievement of Dr. Ian Cree was in actually
completing a prospective randomized trial (discussed elsewhere on this
website). Now if we all could just figure out a way to build upon
his pioneering work in this regard to make some real progress.
Alas, it's not going to be easy...at least here in the USA.
-
Larry Weisenthal
Written (hastily) in hotel room in Bethesda, MD. Sept. 16, 2005