Endostatin Induces Endothelial Cell Apoptosis
Citation
Mohanraj Dhanabal, Ramani Ramchandran, Matthew J. F. Waterman, Hua Lu,
Bertrand Knebelmann, Mark Segal, and Vikas P. Sukhatme
From the Renal Division, Department of Medicine, Beth Israel Deaconess Medical Center and Harvard Medical School,
Boston, Massachusetts 02215
THE JOURNAL OF BIOLOGICAL CHEMISTRY
Vol. 274, No. 17, Issue of April 23, pp. 11721–11726, 1999
© 1999 by The American Society for Biochemistry and Molecular Biology, Inc. Printed in U.S.A.
Received for publication, October 14, 1998, and in revised form, December 17, 1998
Summary
In this study researchers studied the apoptotic effects of endostatin, in endothelial cells and non endothelial cells. Endostatin is a fragment of Collagen XVIII that had been shown to reduce tumor proliferation and migration in mice. Because the process by which this happens was unknown, researchers at Harvard Medical School used four methods to try and track the mechanism by which endostatin increases apoptosis in cells and why it seemed to be endothelial cell specific. They studied cow pulmonary endothelial cells, bovine aortic endothelial cells, bovine adrenal capillary endothelial cells, and several non-endothelial cells including, HUVE, HMVE-L, several fibroblast cells and renal carcinoma cells. In order to study apoptosis, the authors used Annexin V, caspase 3, TUNEL staining, and Western Blot assays with different concentrations of recombinant mouse endostatin added to the various cells and added no endostatin to each cell line as a negative control and added human recombinant tumor necrosis factor as a positive control. In the Annexin assay, apoptosis was detected using a protein that has a high affinity for phosphatidylserine. The authors then used flow cytometry to analyze the percentage of apoptotic cells after various amounts of time had passed. The caspase 3 assay was used to track the activity of the caspase 3, a protein associated with cell apoptosis, in the cells that were introduced to endostatin. Finally, TUNEL staining and Western Blotting were used to detect DNA fragmentation and Bcl-2 and Bax proteins. Using these methods, the authors concluded that endothelial cells treated with endostatin had a rounder morphology associated with apoptosis, had PS moved from the inner membrane to the outside, had increased caspase activity, had increased DNA fragmentation (fig 4), and that Bcl-2 and Bax expression was unchanged (fig 5). From this the authors speculated that endostatin increased apoptosis by reducing the amount of Bcl-2, which is a pro-apoptotic protein that may also interfere with anti-apoptotic proteins such as Bax. Although several cell lines were studied, “the Cow Pulmonary Endothelial cells showed the most dramatic effect” when endostatin was introduced and non-endothelial cells showed none of these signs of apoptosis.
FIG. 4. A, detection of fragmented DNA in adherent C-PAE cells by the TUNEL assay. Adherent cells were fixed with fresh 4% formaldehyde/PBS at 4 °C for 25 min. The cells were permeabilized with prechilled 0.2% Triton X-100/PBS for 5 min on ice. After permeabilization, the TUNEL assay was performed along with propidium iodide dye staining. On staining, pictures were taken immediately using a fluorescent microscope attached to a digital camera and analyzed using the SPOT software. Panels a, c, e, and g are fields of cells stained with propidium iodide (1 mg/ml). Panels b, d, f, and h are the same fields under green fluorescent light. Control cells were incubated in DMEM with 2% FCS. Endostatin concentration in the terminal deoxynucleotidyltransferase1 and terminal deoxynucleotidyltransferase2 samples was 10 mg/ml. TNF-a was added at a final concentration of 20 ng/ml. B, quantitative determination of apoptosis. After TUNEL and propidium iodide staining, the cells were counted in 15 fields for control and endostatin-treated attached cells. For TNFa-treated cells, five fields were counted. The percentage of green divided by the number of red cells in a given field was determined and an average (mean 6 S.E.) of the different fields is presented.
FIG. 5. A, Western blot analysis of C-PAE cell lysate for Bcl-2 protein levels. C-PAE cells were treated with endostatin (10 mg/ml) for the indicated period of time. Total cell lysate from control (2) and treated (1) cultures was analyzed as described earlier. 30 mg of total protein was subjected to SDS polyacrylamide gel electrophoresis analysis followed by Western blot transfer. Immunoblot analysis was performed with antibodies directed against Bcl-2. Reprobing of the same blot with actin antibody was performed to normalize for protein loading. B, immunoblot detection of total cell lysate for Bax expression levels. 30 mg of total cell lysate was separated on 4–15% gradient gel. SDS-polyacrylamide gel electrophoresis analysis was followed by membrane transfer and probing with Bax antibody. Actin probing is shown, as well.
Criticism
The paper is thorough and easy to follow because the descriptions of assays used and procedures followed the same order as in the results. The experiments seem to be well thought out and executed. One thing that stood out to me was that for every negative control, the cells were not only unexposed to endostatin but also all the other buffers used for the assay. Instead, only PBS was added to the controls. Because of this, it can’t be certain that the endostatin is causing the cell apoptosis and not the other buffers used in the experiments. For example, in the caspase 3 assay they added bFGF along with the endostatin to the samples but didn’t add bFGF to the negative control. In the end, the authors were able to use four different assays that detected several different signs of apoptosis to show that endostatin causes apoptosis in cow pulmonary endothelial cells and not in non-endothelial cells.
11 comments:
One thing that stood out to me was that for every negative control, the cells were not only unexposed to endostatin but also all the other buffers used for the assay. Instead, only PBS was added to the controls.
Nice catch!
The authors speculate that endostatin increases apoptosis by reducing the amount of Bcl-2. However, you also say that Bcl-2 and Bax expression was unchanged by the addition of endostatin. Is this really the case (or maybe a typo)?
Could you elaborate on your issue with the buffers used for the negative controls? It seems to me that the same medium (DMEM with FCS, and bFGF) is used in the control and endostatin samples.
The only difference in the negative is that PBS was added to this medium instead of endostatin.
Assuming that Jenna was right and that the concentrations of Bax and Bcl-2 were indeed altered by endostatin, these results are very interesting with respect to Brian's review about taurine's inhibitory affects on apoptosis. Taurine apparently only influences Bcl-2. Perhaps this says something about the pathways that taurine and endostatin take? Everyone seems to only be speculating on Bax...
Just curious, is there a reason why the researchers chose to use bovine/cow cells over mouse cells? I don't know if there are any differences between species, but it might be worth it to check the effects in mouse cells to get comparable data?
It's stated that Bcl-2 is a pro-apoptotic protein that may interfere with anti-apoptotic proteins. How well is Bcl-2 characterized? Maybe its pro-apoptotic qualities play a role in the different results between different cell types?
It is interesting that the authors found that endostatin worked best for cow pulmonary endothelial cells and concluded that endostatin induces endothelial cell apoptosis. Could there be a correlation between endostatin and the type of endothelial cell it affects? Perhaps, endostatin has more affinity for pulmonary endothelial cells.
Jenna and Traci,
That was my mistake. What I meant to write was the Bcl-2 was reduced bu Bax expression remained the same. This result is very much like Brian's paper.
Fergus,
In the Capsase 3 Assay, the paper states that DMEM, FCS, and bFGF is added along with 10 ug/ml endostatin. "For the control plate, only the PBS buffer was added." I'm not sure if I'm reading this wrong, but I took this to mean that they only added PBS to the control plate.
Michelle,
I think they used Cow cells because endostatin had already been shown to regress tumors in mice so they wanted to see its effects on other cells but that is just a guess. I believe Bcl-2 is fairly well characterized because I have seen a lot of papers on it and they all seem to agree that it is pro-apoptotic. They have also been studied in many different types of cells (see Brian's Post).
Karthik,
The paper states that the mechanism of endostatin is unknown but that it has been shown to have no effect on non-endothelial cells. The paper however, doesn't discuss its effects on different types of endothelial cells. It maybe have more effect on pulmonary ones.
Good job catching the problem with their negative controls!
I did some research, and I noticed that endostatin is also an angiogenesis inhibitor (I'm assuming because of this very reason of inducing endothelial cell apoptosis, and therefore inhibiting blood vessel growth since vessels require primarily endothelial cells). Interestingly, many companies/groups have tried using endostatin as an anticancer therapy, but it hasn't been very efficient due to its short half-life. However, there are some groups trying to work around this problem by altering endostatin synthetically.
Just an interesting tidbit that I thought I'd share.
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