1 Department of Pathology and
2 Department of Obstetrics and Gynecology, Columbia University, College of Physicians and Surgeons, 630 West 168th Street, New York, NY 10032 and
3 Department of Pathology, Weill Medical College of Cornell University, 1300 York Avenue, New York, NY 10021, USA
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Abstract |
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Introduction |
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The APC encoding locus on chromosome 5q21 shows loss of heterozygosity (LOH) in ~25% of breast cancers (10). Frequent alterations in expression of E-cadherin and - and ß-catenins have been reported in a survey of 18 human breast cancer cell lines (11). High Wnt gene expression (Wnt-2, Wnt-4, Wnt-7b) has been seen in human proliferative breast lesions (12). Overexpression of Wnt-1 and Wnt-3 in the murine mammary gland induces mammary hyperplasia and increases the incidence of mammary gland tumors (1). In addition, APCmin mice, which represent a model for the human FAP syndrome, have an increased incidence not only for intestinal neoplasias but also for mammary tumors (13). Despite the link between Wnt signal activation and mammary gland tumors in the mouse, comparable signal activation due to mutations in genes encoding Wnt signaling components has not been documented in human breast cancer. In the present study, we screened a panel of 27 cell lines, either derived from human breast carcinomas or established by immortalization of normal breast epithelial cells, for alterations in the ß-catenin,
-catenin and APC proteins and for mutations in the APC, ß- and
-catenin genes.
Cell lines BT 20, BT 474, BT 483, BT 549, CAMA 1, DU 4475, HBL 100, HS 578 T, MCF7, MCF10A, MDA-MB 157, MDA-MB 175 VII, MDA-MB 231, MDA-MB 330, MDA-MB 361, MDA-MB 415, MDA-MB 435S, MDA-MB 436, MDA-MB 453, MDA-MB 468, SKBR 3, T 47 D, UACC 812, UACC 893, ZR 75-1 and ZR 75-30 were purchased from the American Type Culture Collection (ATCC; Rockville, MD). MCF10A is a spontaneously immortalized line from normal human breast epithelial cells, and HBL 100 is an SV40 immortalized human breast epithelial cell line. HB2, another SV40 immortalized human breast epithelial cell line, was obtained from Dr Joyce Taylor-Papadimitriou (London, UK). Cells were grown under recommended conditions and harvested at 90100% confluency. For total cell protein extraction, cells were lysed in TENT buffer (50 mM Tris pH 8.0, 1 mM EDTA, 150 mM NaCl, 1% Triton X-100), centrifuged, the supernatant admixed with protein sample buffer and boiled. Cytosolic and membranous fractionation was carried out as described previously (3). Total protein (30 µg) was separated by electrophoresis on 8% SDSpolyacrylamide gels, transferred onto nitrocellulose (Micron Separations Inc., Westboro, MA) and identified using primary antibodies against ß- and -catenin (Transduction Laboratories, Lexington, KY), and chemiluminescence detection (ECL; Amersham, Arlington Heights, IL). To screen for mutations in exon 3 of the ß- and
-catenin genes, a portion of that exon was amplified from genomic DNA from all cell lines using the following primer pairs: ß-catenin, Forward(F) 5'-ATTTGATGGAGTTGGACATGGC-3' and Reverse(R) 5'-GAGGAAGAGGATGTGGATACCTCC-3';
-catenin, F 5'-AGCCACGATGGAGGTGATGAAC-3' and R 5'-CCTGGGTGTAAGTGGTGGTTTTC-3'.
To analyze the entire ß-catenin gene from DU4475, cDNA was synthesized in 12 separate RTPCR reactions (primer sequences available upon request) using total RNA as template. cDNA was then PCR-amplified, submitted to automated sequencing and compared to the published ß-catenin sequence (14). To screen breast cancer cell lines for truncation mutations in APC, the TNT® coupled reticulocyte lysate system (Promega, Madison, WI) was used, following the manufacturer's instructions. Two overlapping segments of the APC gene, spanning the region from codon 686 to 1693, were amplified from cDNA using the following T7-modified primers (T7-trans = GGATCCTAATACGACTCACTATAGGGAGACCACCATGG): segment A (codons 686-1217 ), F 5'-T7-transATGCATGTGGAACTTTGTGG-3' and R 5'-GAGGATCCATTAGATGAAGGTGTGGACG-3'; segment B (codons 10991693), F 5'-T7-transTTTCTCCATACAGGTCACGG-3' and R 5'-GGAGGATCCTGTAGGAATGGTATCTCG-3'.
Aliquots of 5 µl of the in vitro transcription/translation reaction were separated on 420% TrisHCl SDSpolyacrylamide gels (Ready Gel®; Bio-Rad, Hercules, CA) and the product visualized by autoradiography (BioMax Kodak, Rochester, NY). Segment B of the APC gene in cell line DU 4475 was sequenced using the Thermo Sequenase® kit (Amersham, Arlington Heights, IL). Additional primers (sequences available upon request) were obtained from Operon Technologies Inc. (Alameda, CA). An aliquot of 2 µl of the chain-termination reaction products were submitted to electrophoresis on a CastAway® sequencing device (Stratagene, La Jolla, CA) using precast 6% polyacrylamide7 M urea gels and visualized by autoradiography (BioMax; Kodak, Rochester, NY). All experiments were performed at least twice.
Total cell lysate western blot analysis (Figure 1) showed strong expression of ß-catenin in BT 20, BT 474, BT 483, BT 549, DU 4475, HB2, HBL 100, HS 578 T, MCF7, MCF10A, MDA-MB 157, MDA-MB 175 VII, MDA-MB 231, MDA-MB 361, MDA-MB 415, MDA-MB 468, T 47 D, UACC 893, ZR 75-1 and C57-Wnt-1 (positive control); weak expression was seen in CAMA 1, MDA-MB 435 S, MDA-MB 436, MDA-MB 453 and UACC 812; ß-catenin was detected at very low levels in MDA-MB 330, SKBR 3 and ZR75-30. In DU 4475, ß-catenin expression was extremely strong, exceeding the positive control (Figure 1A
). In MDA-MB 468, a double band was seen with a second signal at ~80 kDa (Figure 1A
).
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On the basis of these results, the following cell lines were selected for analysis of cytosolic (Figure 2) and membranous protein fractions (data not shown): CAMA 1 (weak expression of ß-catenin), DU 4475 (high expression of ß-catenin), HS 578 T (low levels of
-catenin), MDA-MB 468 (ß-catenin double band), SKBR 3 (low levels of ß-catenin) and HB2 (control). As expected, in most lines ß- and
-catenin levels were very low in the cytoplasmic fraction (Figure 2
), whereas both proteins were prominent in the membranous fraction (data not shown). Of the cell lines analyzed, ß-catenin was significantly elevated in the cytosolic fraction of DU 4475 (Figure 2
).
-Catenin levels were slightly stronger in the cytosolic fraction of DU 4475, as compared with the other cell lines analyzed, but not to the extent exhibited for ß-catenin. Low levels of ß-catenin in CAMA 1 (Figure 1
) were confirmed in the fractionated analysis (Figure 2
).
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The protein truncation assay was performed on two APC segments encompassing codons 686 through 1693 for all cell lines listed except HB2, MCF10A, MDA-MB 330 and MDA-MB 435S. Of all protein products, one showed an aberrant size: The segment B product from DU 4475 had an apparent molecular weight of 70 kDa instead of the expected 100 kDa (Figure 3A). No wild-type allele, or full length protein product, was detected in this cell line (Figure 3A
). Sequencing of the respective APC gene segment revealed a point mutation at position 4747 of the coding sequence (G
T), converting codon 1577 into a stop codon (E1577stop) (Figure 3B
).
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The APC mutation reported here (E1577stop), has not been described previously (based on the Human Gene Mutation Database, http://www.uwcm.ac.uk/uwcm/mg/hgmd0.html ,as of March 6, 2000). It is located at the end of the MCR, in the domain containing seven phosphorylation-dependent ß-catenin binding sites and results in a protein lacking the basic region, the microtubule, DLG and EB1 binding domains (7). Although studies have shown that loss of heterozygosity at the APC site on chromosome 5q21 occurs in up to 38% of primary breast cancers (18,19) only two mutations of the APC gene have been reported, both are point mutations leading to amino acid substitutions (18). In addition, an APC mutation in a primary breast cancer has been reported (20), but no documentation of alterations in ß-catenin levels was presented.
The DU 4475 cell line was derived from a recurrent thoracic wall tumor following mastectomy for a poorly differentiated invasive ductal breast carcinoma in a postmenopausal patient (21). DU4475 cells are highly transformed and do not adhere to the culture dish, but rather grow in suspension. It is not clear whether upregulation of ß-catenin contributes to these growth characteristics. Since APC mutations are rare in breast cancer, we considered the possibility that this mutation was acquired in culture. In our analysis, there was no evidence of a second normal allele. This is interpreted as a hemizygous loss of the other allele since homozygosity for a point mutation would be extremely unlikely. Presumably, the point mutation in one allele (Figure 3B) was complemented by loss of the other allele (Figure 3A
). The acquisition of these two independent mutations is unlikely to occur during propagation in vitro; although it cannot be formally excluded. There is no evidence from the original description (21) that the patient had FAP, suggesting a germline APC mutation.
The variability of expression levels of ß- and -catenin in the other lines may represent the normal range of variation. Alternatively, it may be due to translational and post-translational influences or mutations in other regions of the respective genes. Our results of ß- and
-catenin expression are largely concordant with other reports (11,22). The significance of minor deviations [in contrast to Pierceall et al. (11) we found strong ß-catenin expression in BT 474, MCF7, MDA-MB 231, MDA-MB 468 and ZR 75-1] is uncertain. Concurring with our results, a study of 11 breast carcinomas revealed no mutations in exon 3 of the
- or ß-catenin genes by RTPCR and single strand conformation polymorphism (SSCP) analysis (23).
In conclusion, we screened 27 human cell lines derived from breast carcinomas or immortalized breast epithelial cells for alterations in the downstream elements of the Wnt signaling pathway; APC, ß- and -catenin. We report the first APC mutation with associated ß-catenin upregulation in a human breast carcinoma cell line (DU 4475). Unlike colon carcinomas and melanomas, however, deregulation of the Wnt signaling pathway does not seem to be a frequent event in human breast carcinomas.
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Notes |
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Acknowledgments |
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References |
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