(Received for publication, April 11, 1997, and in revised form, May 13, 1997)
From the Division of Growth Regulation, Department of Medicine, Beth Israel Deaconess Medical Center, Harvard Medical School, Boston, Massachusetts 02215
Pleiotrophin (PTN) is a recently described 18- kDa heparin binding growth/differentiation factor. It also is a proto-oncogene; cells transformed by the Ptn gene form highly angiogenic tumors when implanted into the nude mouse. PTN may be an important regulator of transformation in other tumors, because constitutively high levels of expression of the pleiotrophin (Ptn) gene are found in human breast cancer and other malignant cell lines, and its levels of expression are high in many human tumor specimens. To determine whether PTN is an important regulator of the malignant phenotype of human breast cancer cells, we constructed a mutant cDNA to encode a truncated PTN designed to heterodimerize with the product of the endogenous Ptn gene during processing. The mutant gene product blocked transformation of NIH 3T3 cells by the wild type (wt) Ptn gene product. The mutant Ptn cDNA was then introduced into human breast cancer MDA-MB-231 cells, and clonal lines that stably express the mutant Ptn cDNA were selected. The truncated PTN was shown to form heterodimers with the endogenous Ptn gene product in these cells. Furthermore, the MDA-MB-231 cells that express the mutant Ptn gene were no longer transformed; they failed to form plaques or colonies in soft agar and were unable to form tumors in the athymic nude mouse. The results establish an important role of PTN in the dysregulated growth of human breast cancer cells and suggest that constitutive expression of PTN may be essential to the malignant phenotype of human breast cancers in vivo.
Pleiotrophin (PTN)1 is an 18-kDa heparin-binding protein that was purified from bovine uterus and from neonatal rat brain (1, 2). The Ptn cDNA (3, 4) encodes a lysine-rich, highly basic protein of 168 amino acids with a 32-amino acid signal sequence that is highly conserved in bovine, rat, human, and chicken (3, 5). PTN exhibits nearly 50% amino acid sequence identity and perfect conservation of 10 cysteine residues with the protein product of Mdk, a gene expressed in the early stages of retinoic acid-induced differentiation of mouse embryonal carcinoma cells (6), and with RI-HB, a protein isolated from chick basement membranes (7), linking Ptn with Mdk as a member of a new family of developmentally regulated genes (3). PTN promotes cell growth of NIH 3T3 and NRK fibroblasts (1, 3), endothelial cells (8-10), epithelial cells (9, 11), and osteoblasts (12-14). It induces neurite outgrowth from neuronal cells (1, 2) and process outgrowth from oligodendrocyte progenitors (15) and is angiogenic in the rabbit corneal pocket assay (8), suggesting that PTN may have a central role in regulating growth of cells of different lineages and organ systems.
The importance of PTN in malignant cell growth was first established when introduction of the exogenous Ptn gene into NIH 3T3 and NRK cells led to morphological transformation, anchorage independent growth, and tumor formation with significant neovascularization in vivo in the nude mouse (16). It was shown subsequently that SW13 cells transformed by Ptn also develop highly vascular tumors in the flanks of athymic nude mice (9), that high levels of the Ptn gene are expressed in specimens of many human tumors, including neuroblastoma, glioblastoma, prostate cancer, lung cancer, and Wilms' tumor, and that many breast cancer cells and about one-fourth of over 40 human tumor cell lines of different origins also express the Ptn gene in significant levels (9, 17, 18). These findings, strengthened by observations that the transformed phenotype of human melanoma cells (WM852) can be suppressed specifically by Ptn-targeted ribozymes (19, 20), strongly support the view that PTN has a central regulatory role in neoplastic cell growth. To directly test the role of PTN in human tumor cell lines, we constructed a mutant Ptn cDNA to encode a truncated PTN designed to heterodimerize with the wt Ptn gene during processing and thus to act as a dominant negative effector of PTN.
In this manuscript, we establish that expression of the truncated PTN prevents transformation of NIH 3T3 cells by wt PTN and that the mutant PTN forms heterodimers with PTN itself. We then demonstrate that expression of the truncated PTN reverts the transformed phenotype of clonally selected human breast cancer (MDA-MB-231) cells that constitutively express significant levels of the endogenous Ptn gene. The results establish that high levels of expression of PTN appear to be essential to maintain the transformed phenotype of MDA-MB-231 cells and that the Ptn gene may be a central regulator of the dysregulated growth of many human tumors.
A 345-base pair (bp)
cDNA fragment containing 111-bp 5-untranslated sequences and the
sequences to encode mouse PTN residues
32 to +40 was fused in frame
with an 18-bp DNA fragment encoding 6 histidine residues and cloned
into the PstI/XbaI site downstream from the pGK
promoter of the eukaryotic expression vector pPGK-Neo-bpA (21). The
resultant plasmid was designated pMMutPtn-1. The human wild
type (wt) Ptn expression vector, pHuPtn,
containing a full-length human Ptn cDNA fragment, was
cloned into the KpnI/EcoRI site of pAGE103 vector
driven by SV40 promoter as described previously (16). Amino acid
residues 1-40 (after cleavage of the signal peptide) of mouse and
human PTN are identical, and thus the truncated PTN is equally
effective in mouse and human lines.
Mouse NIH 3T3 and human breast cancer (MDA-MB-231) cells were maintained in Dulbecco's modified Eagle's medium supplemented with 10% bovine calf serum and 10% fetal bovine serum, respectively. 1 × 106 cells per dish were plated on 100-mm culture dishes 20 h before transfection with 15 µg of pHuPtn plus 15 µg of pBluescript II, 15 µg of pMMutPtn-1 plus 15 µg of pHuPtn, or 15 µg of the empty pAGE103 vector plus 15 µg of pBluescript II into NIH 3T3 cells as indicated, using a modified calcium phosphate precipitation technique (22). Cells were transfected on three separate occasions with DNA from three separate extractions. The results were effectively the same. After 3 days, cells were selected with neomycin (Life Technologies, Inc.) at 700 µg/ml, and media were changed every 3 days until foci appeared. Cells from established foci were pooled and subsequently assayed by focus formation and growth in soft agar.
MDA-MB-231 cells were transfected with the Lipofectin method (23) and selected with G418 at 500 µg/ml. Media were changed every 3 days until colonies formed. These clonal cell lines were selected by mechanical agitation, expanded for later use, and designated HBC (human breast cancer) Ptn1, -2, and -3. The controls that lacked the Ptn mutant constructs ("empty" vector) were designated as HBC vector 1, 2, and 3.
Northern Blot AnalysisTotal RNA was isolated by the
guanidinium-thiocyanate method (24). Twenty µg of total RNA (20 µg)
was separated on 1.2% formaldehyde-agarose gels, blotted onto nylon
membranes (Hyclon, Micron Separations, Westboro, MA), prehybridized,
and hybridized with an [-32P]dCTP-labeled
SmaI fragment of mouse Ptn cDNA. After
overnight hybridization, blots were washed twice with 0.5 × SSC
and 0.1% SDS for 20 min at room temperature and once for 20 min at
68 °C and autoradiographed with intensifying screens at
70 °C.
To detect heterodimers of mutant PTN and wt PTN, clonally selected MDA-MB-231 cells that harbored pMMutPtn-1 or vector alone were lysed in 0.8 ml of cell lysis buffer (10 mM Hepes, pH 7.2, 142.5 mM KCl, 1 mM EGTA, 5 mM MgCl2, and 0.5% Nonidet P-40) per 100-mm dish for 30 min. After centrifugation, 25 µl of Ni-NTA Sepharose beads (Qiagen) were added to the supernatants, incubated at 4 °C for 24 h, washed 3 times with Tris-buffered saline containing 0.1% Tween 20 (TBST, pH 7.35), and eluted with 15-30 µl of SDS-gel loading buffer. Eluates were separated by 12.5% SDS-polyacrylamide gel electrophoresis, transferred to Immobilon membranes (Millipore), immunoblotted with an anti-histidine "tag" monoclonal antibody (1:250, Novagen), and visualized by the ECL system (Amersham) according to the manufacturer's instructions. To test whether the PTN mutant protein forms heterodimers with wild-type PTN of MDA-MB-231 cells, the same blot was stripped and probed with a chicken anti-human PTN antibody under the same conditions as above to establish that the human wt PTN molecule was isolated with the truncated mutant PTN using the affinity isolation technique specific for the His-tagged mutant PTN.
AntibodiesChicken anti-human PTN antibodies were prepared using recombinant human PTN expressed in Escherichia coli as antigen and purified as described (1). It is used at a dilution of 1:500.
Focus Formation, Soft Agar Assay, and Tumor Formation in Nude MiceFor focus formation assays, 2 × 105 NIH 3T3 cell transfectants were pooled and plated in triplicate onto 60-mm dishes. Media were changed every 3 days. After 16 days, cultures were stained with crystal violet, and the foci on each dish were photographed and counted. To test anchorage-independent growth on soft agar, 5 × 104 cells from the pooled NIH 3T3 or clonally selected MDA-MB-231 cell lines were suspended in 5 ml of agar containing Dulbecco's modified Eagle's medium, 10% calf serum or 10% fetal calf serum and were overlaid over 0.7% agar in two 60-mm dishes. After 16 days, colonies with more than 20 cells were scored as positive using an inverted microscope equipped with a measuring grid.
For tumor formation, female athymic nude mice (Ner nu/nu; Harlan Sprague Dawley, Indianapolis, IN) were injected subcutaneously in each flank with 2 × 106 cells from the above 6 clonally selected cell lines, and tumor size was measured daily, starting at 10 days following the injections.
PTN contains 10 cysteine
residues that establish intramolecular disulfide bonds (25). We
therefore constructed a mutant cDNA (pMMutPtn-1) to
encode mouse PTN amino acid residues 32 to +40 that likely would
establish non-functional heterodimers with the product of the wt
Ptn cDNA (wtpHuPtn) after cleavage of the
signal sequence and tested the ability of the mutant cDNA product
to inhibit transformation of NIH 3T3 cells by PTN. Northern blots
established that the NIH 3T3 cells that were transfected with wt
pHuPtn alone or with wt pHuPtn and
pMMutPtn-1 expressed both genes at essentially equal levels
(data not shown).
Cells that were co-transfected with wt pHuPtn and pMMutPtn-1 together were normal in appearance and growth rate. The growth characteristics and appearance of these cells did not differ from cells transfected with the empty vector or from non-transfected NIH 3T3 cells. In contrast, cells transfected with the wt HuPtn construct alone were typically transformed; they had a higher growth rate and were clustered, highly refractile, and spindle-shaped in appearance. At confluence, these cells grew to a density ~2-fold higher than the cells co-transfected with the wt HuPtn and pMMutPtn-1 plasmids together or cells co-transfected with the empty vector alone.
Cells that were transfected with the wt HuPtn construct had readily detected foci after 16 days. However, the number of foci was dramatically reduced in NIH 3T3 cells co-transfected with both the wt HuPtn and pMMutPtn-1 constructs as scored in Table I. However, when lysates were prepared from the foci that developed from cells that were co-transfected with wt and mutant Ptn constructs and analyzed in Northern blots, transcripts of the exogenous Ptn mutant gene were not detected (data not shown), indicating that the mutant gene was not expressed at detectable levels. Although these foci were scored as observed, a (0) was placed after the number of foci observed in Table I to indicate that in the foci examined by Northern blots, the mutant Ptn transcripts were not detected; it is presumed that these foci arose from clonally selected cells that express the neomycin resistance gene and the wt Ptn cDNA but failed to express the mutant Ptn cDNA.
|
In soft agar assays, expression of the mutant Ptn gene also effectively prevented transformation by the wt Ptn gene (Table I). When colonies that arose from the clonally selected cells transfected with both wt Ptn and mutant Ptn cDNAs were analyzed by Northern blots as above, in no instance were transcripts of the mutant Ptn cDNA detected. These colonies were scored as observed; the (0) following the number of colonies indicates that in the colonies tested, none expressed the mutant Ptn cDNA in detectable levels.
The data suggest that the truncated PTN product of pMMutPtn-1 functions as a true dominant negative effector of PTN and establish that PTN-dependent transformation in both focus and colonary formation assays is effectively prevented by expression of the Ptn mutant cDNA to encode PTN residues 1-40.
The Dominant Negative PTN Effector Reverses the Malignant Phenotype of MDA-MB-231 Cells in Culture and in VivoMDA-MB-231 cells are
derived from a highly malignant human breast cancer and constitutively
express the endogenous Ptn gene in high levels (9), raising
the important question whether the endogenous Ptn gene and
the PTN signaling pathway have an important regulatory role in the
aggressive growth of these cells. To test the mutant Ptn
gene construct in this highly transformed cell line, we introduced
pMMutPtn-1 into MDA-MB-231 cells and isolated, expanded, and
analyzed G418-resistant clones by Northern blots (Fig.
1A). The exogenous Ptn mRNA
(~1.0 kilobase) is easily differentiated from the endogenous
Ptn mRNA (1.5 kilobases). Clones HBC Ptn-1
and HBC Ptn-2 express high levels of the mutant Ptn gene whereas it was not detected in HBC Ptn-3
or in cell lines that harbor the pGK-Neo-pbA vector alone (HBC vectors
1, 2, and 3). Since the mouse PTN mutant protein was fused with a
six-histidine "tag" at its C terminus, the mutant protein is
readily detected with a His-tag monoclonal antibody. As shown in Fig.
1B, only HBC Ptn-1 and HBC Ptn-2
expressed the mutant PTN protein. Clones transfected with the neomycin
resistance gene alone and clone HBC Ptn-3, which failed to
express the mutant Ptn gene, also failed to express the
protein in Western blots probed with the anti-6× histidine tag
monoclonal antibody.
All six of the clonally selected, stably transfected MDA-MB-231 cells were expanded and placed in soft agar. Cells harboring pMMutPtn-1 and pMMutPtn-2 formed substantially fewer colonies in soft agar (Table II). These colonies also were substantially smaller than colonies of HBC Ptn-3 in soft agar. The results indicate that the dominant negative PTN effector greatly attenuates focus formation and anchorage-independent growth of MDA-MB-231 cells and suggest that the PTN signaling pathway has an important and perhaps essential regulatory role in the ability of these human tumor cells to sustain the transformed phenotype.
|
The clones that stably express mutant PTN-(1-40) were also tested for their ability to form tumors in the nude mouse. The two clones that expressed the mutant PTN-(1-40) protein at high levels (HBC Ptn-1 and HBC Ptn-2) were compared with HBC Ptn-3 cells and with cells expressing vector alone (HBC vector 1, 2, and 3); after 6 weeks, tumors at the sites of injection of MDA-MB-231 cells that express mutant PTN-(1-40) were strikingly smaller than tumors in animals injected with control MDA-MB-231 cells that stably express the neomycin gene alone (Table II). These results indicate that the ability of MDA-MB-231 cells to form tumors in vivo in the nude mouse is markedly attenuated by the dominant negative PTN effector. The results confirm the results of the tumorigenic assays in soft agar and argue strongly that in MDA-MB-231 cells, PTN has a central regulatory role in maintaining the transformed phenotype in vivo.
Heterodimers of wt PTN and PTN Mutant 1-40 Were Detected in pMMutPtn-1 Stably Transfected MDA-MB-231 CellsFully processed
PTN is a monomer with internal cysteine residues 15 and
44,
23
and
53,
30 and
57,
67 and
99, and
77 and
109 linked as
disulfide bonds (25). The dominant negative cDNA construct was
designed to encode residues
32 to +40. There are 3 cysteine residues
(+15, +23, +30) in the truncated PTN product; it was anticipated that
these residues would dimerize with the wt Ptn gene product
during processing.
To determine if the mutant PTN protein establishes heterodimers with wt
PTN in MDA-MB-231 cells that stably express the mutant Ptn
gene, cell lysates were incubated with Ni-NTA to "capture" the
His-tagged PTN mutant, and eluates were prepared and analyzed by
Western blotting with chicken polyclonal anti-human PTN
antibodies.2 The chicken polyclonal
anti-human PTN antibody recognized the endogenous (wt) PTN in lanes in
which lysates of HBC clones Ptn-1 and Ptn-2 were
analyzed (Fig. 2). When the membranes used in Western blotting were stripped and reprobed with the anti-His tag antisera, the
truncated PTN (data not shown) was recognized as well, indicating that
the Ni-NTA captured both the mutant His-tagged truncated PTN and the wt
PTN together. As anticipated, endogenous (wt) PTN was not
"captured" with the His-tagged PTN mutant in lysates of HBC
Ptn-3 or lysates of the control HBC vector 1, 2, and 3 cells, suggesting that the Ni-NTA column effectively captured the
His-tagged mutant PTN as a heterodimer with wt PTN. These results thus
indicate that the His-tagged mutant PTN-(1-40) associates with wt PTN
to form heterodimers in MDA-MB-231 cells and suggest that the mechanism of the dominant negative effect of the truncated PTN-(1-40) is the
formation of non-functional heterodimers with wt PTN.
The data demonstrate that the mutant Ptn cDNA to
encode PTN residues 32 to +40 functions as a dominant negative
effector of wt PTN. The mutant PTN-(1-40) effectively prevents
transformation of NIH 3T3 cells by wt PTN and effectively reverses the
malignant phenotype of the human breast cancer MDA-MB-231 cell line
that constitutively expresses high levels of the endogenous
Ptn gene. Finally, the data establish that mutant
PTN-(1-40) forms heterodimers with wt PTN, suggesting that the
mechanism of the dominant negative effect of PTN-(1-40) is to
establish non-functional complexes presumably through disulfide
interactions with wt PTN during processing. Because Mdk retains perfect
conservation of cysteine residues with PTN (3), it may also be possible
for Mdk to heterodimerize with the truncated PTN and be inactivated
through heterodimerization. To further establish the specificity of the
mutant PTN for PTN itself in MDA-MB-231 cells, Northern blots were
prepared and Mdk transcripts were not found (data not shown). This
result is consistent with published experiments that established a
negative correlation of the levels of expression of the Mdk
gene as rat mammary tumors progress in malignancy (26).
The most important conclusion of this work is the dependence of a highly malignant human breast cancer cell line on the constitutive high expression of PTN and PTN-mediated signal transduction to maintain the transformed phenotype in culture and in vivo. The ability to block transformation with the dominant negative mutant suggests a central role of the PTN signaling system in tumorigenesis and supports the contention that this signaling system may be a major regulator of neoplastic transformation in the highly malignant MDA-MD-231 human breast cancer cell line. The results suggest that expression of the Ptn gene and its signaling pathway in appropriately high levels may play a crucial regulatory role in many neoplasms of diverse origins. This potentially highly important regulatory role of PTN in transformation is consistent with previous results that established that the Ptn gene itself directly transforms NIH 3T3 cells (16) and that a Ptn ribozyme construct reverses transformation of human melanoma cells in culture (19, 20). In addition to breast cancer, Ptn mRNA is also highly expressed in a large number of samples of other human tumors including neuroblastoma, glioblastoma, prostate cancer, lung cancer, and Wilms' tumor, and in over 10 tumor cell lines derived from human tumors (9, 17, 18). The identification of PTN and its signaling pathway as an important regulator molecule that is specific and crucial for solid tumor progression in vivo suggests a number of strategies for clinical applications in which PTN is a promising target for the development of specific anti-tumor drugs.
We gratefully acknowledge the expertise of Mary Ann Strileckis in the preparation of this manuscript.