This Article Abstract Full Text (PDF) Alert me when this article is cited Alert me if a correction is posted Services Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Llor, X. Articles by Tyner, A. L. Search for Related Content PubMed PubMed Citation Articles by Llor, X. Articles by Tyner, A. L.

BRK/Sik Expression in the Gastrointestinal Tract and in Colon Tumors¹

Departments of Molecular Genetics and Medicine, University of Illinois College of Medicine, Chicago, Illinois 60607

	ABSTRACT

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Clones encoding the breast tumor kinase BRK were isolated from a normal human small intestinal cDNA library that was screened with the cDNA encoding the mouse epithelial-specific tyrosine kinase Sik. Although BRK and Sik share only 80% amino acid sequence identity, Southern blot hybridizations confirmed that the two proteins are orthologues. Sik was mapped to mouse distal chromosome 2, which shows conservation of synteny with human chromosome 20q13.3, the location of the BRK gene. BRK expression was examined in the normal gastrointestinal tract, colon tumor cell lines, and primary colon tumor samples. Like Sik, BRK is expressed in normal epithelial cells of the gastrointestinal tract that are undergoing terminal differentiation. BRK expression also increased during differentiation of the Caco-2 colon adenocarcinoma cell line. Modest increases in BRK expression were detected in primary colon tumors by RNase protection, in situ hybridization, and immunohistochemical assays. The BRK tyrosine kinase appears to play a role in signal transduction in the normal gastrointestinal tract, and its overexpression may be linked to the development of a variety of epithelial tumors.

	INTRODUCTION

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Sik is an intracellular tyrosine kinase that was identified in a screen for tyrosine kinases in intestinal epithelial cells (1) . Although it is related to the SRC family and contains SH2 and SH3 domains, it has a very short unique NH₂ terminus and is not myristoylated (2) . Expression of Sik is restricted to epithelial cells and has been detected in the skin and in all linings of the alimentary canal. Transcription of Sik is initiated as cells migrate away from the proliferative zone and begin the process of terminal differentiation. Sik expression is first detected at mouse embryonic day 15.5 in the differentiating granular layer of the skin (2) .

The role of Sik in differentiation was examined in mouse keratinocytes (3) . The addition of calcium to cultured mouse keratinocytes induces a terminal differentiation program and a cascade of tyrosine phosphorylation. Sik was activated within 2 min after calcium addition to keratinocytes. It was found to bind a rapidly phosphorylated M_r 65,000 GAP⁵ -associated protein (GAP-A.p65) through its SH2 domain. Overexpression of Sik in the embryonic mouse keratinocyte cell line resulted in increased expression of the differentiation marker filaggrin during calcium-induced differentiation. This suggested that Sik, the only known tyrosine kinase activated in keratinocytes within minutes after calcium addition, is involved in a signal transduction pathway that may promote differentiation.

Here we demonstrate that the breast tumor kinase BRK is the human orthologue of Sik. A portion of the BRK catalytic domain was initially cloned using PCR and degenerate primers corresponding to the conserved regions of tyrosine kinase catalytic domains and RNA isolated from involved axillary nodes from a patient with metastatic breast cancer. The full-length BRK cDNA was isolated from the MCF-7 and T-47D breast cancer cell lines (4) . BRK has been detected in breast tumors and in a number of breast tumor cell lines, but not in normal breast, liver, placenta, pancreas, or other tissues (4 , 5) . Of 41 primary breast tumor samples quantified by Western blotting relative to cytokeratin 18, BRK was overexpressed 5-fold or more in 27% of the samples and overexpressed 2-fold or more in 61% of the samples as compared to normal breast tissue. One tumor expressed 43-fold higher levels of BRK protein (5) .

BRK has also been cloned from melanoma cells and named PTK6 (6) . BRK mRNA levels were undetectable in seven primary melanoma lines, two normal samples of melanocytes, and in biopsies from metastatic melanomas. However, BRK was present in 2/22 metastatic melanoma cell lines, and may be expressed in 10% of primary melanoma and melanocyte cultures (7) .

Using human/hamster somatic cell hybrids, BRK was mapped to human chromosome 20 (6) . Fluorescence in situ hybridization was used to further localize the BRK gene to 20q13.3 (8) . 20q13.3 was one of five regions found to be amplified in homogeneously staining regions of chromatin of three primary breast carcinomas (9) . In addition to being amplified in breast tumors and breast tumor cell lines (10 , 11) , amplification at 20q13 has been detected in other epithelial tumors including gastric and gastro-esophogeal tumors (12) and colon tumors (13) . We discuss the relationship between BRK and Sik and the possible role that this kinase may play in epithelial cell cancers.

	MATERIALS AND METHODS

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Isolation and Characterization of cDNA Clones.
A human small intestine (duodenum) 5' Stretch cDNA library prepared in the gt11 vector (Clontech) was screened using a ³²P-labeled 562-bp SstI fragment of the Sik cDNA (2) . cDNA clones were sequenced by the dideoxynucleotide chain termination method (14) , using Sequenase (USB).

Tissue and Blood Samples.
Tissues for in situ hybridization experiments were surgically resected, fixed in neutral buffered formaldehyde, and embedded in paraffin. Tissues for protein expression studies were obtained through pinch biopsies obtained during endoscopic procedures performed in the GI suite at the University of Illinois Hospital (Chicago, IL). All samples were collected after informed consent was obtained in accordance to the previously approved institutional review board protocol.

Southern Blot Analyses.
Human genomic DNA was prepared from a blood sample obtained from a healthy volunteer. Mouse genomic DNA was extracted from the liver of a CD1 mouse. Ten µg of human and mouse DNA were digested with BamHI, HindIII, SstI, and BamHI-HindIII; subjected to electrophoresis through a 0.8% agarose gel; and transferred to a nitrocellulose membrane. Probes for hybridization included a 562-bp purified SstI fragment of Sik cDNA and an 884-bp SacI-EcoRI fragment of human BRK cDNA. 100 ng of each fragment was used for random primer labeling with 50 µCi of [³²P]dCTP. Membranes were washed in 0.1% SDS and 0.1x SSC at 65°C for the corresponding species probe and at 55°C for the interspecies hybridizations and exposed to film.

Mapping of Mouse Sik.
Sik is closely linked to Eef1a2 and was found on BAC clones containing this gene. Mapping of Eef1a2 was carried out using DNA from The Jackson Laboratory Interspecific Backcross BSS panel (15) . This panel is made up of 94 N2 offspring derived from the cross (C57BL/6J x SPRET/Ei)F₁ x SPRET/Ei. Over 3310 loci have been mapped in this cross. Eef1a2 mapped to within the most distal group of markers on mouse chromosome 2. A BAC library constructed from 129/Sv ES cell DNA (Research Genetics) was screened with primers corresponding to Eef1a2. Two independent clones were isolated, each containing an insert of approximately 65–70 kb. Sequencing indicated that each clone contained the coding and 3'-UTR sequence of the Sik gene in addition to Eef1a2. One clone also contained the 5'-UTR sequence of Sik.

Sequences compared in Fig 3B include mouse sequences Pltp: basepairs 67-1548 of GenBank locus U37226 (NCBl accession 1051265); Eya2: 166-1587 of U81603 (1816530); Gnas: 20-1204 of Y00703 (51127); Pck1: 1-546 of EST sequence AI037119, 470-539 of AA562908, 1-59 of AI021099, 18-478 of AA080172, 458-569 of AA286042, 9-537 of AA106463, 118-515 of AA110781; Lama5: 5906-10820 of U37501 (2599231); Eef1a2: 134-1525 of L26479 (1220409); Col9a3: 1-333 of X91012 (975686), 1-104 of AA027742 (1493761); Sik: 286-1641 of U16805 (847794); human sequences PLTP: 88-1569 of L26232 (468325); EYA2: 196-1617 of Y10261 (1834488); GNAS: 69-1253 of X04408 (31914); PCK1: 122-1990 of L05144 (189944) excluding 589-609 (for which mouse EST sequence was unavailable); LAMA5: 1-4930 of AB011105 (3043589); EEF1A2: 84-1475 of X70940 (38455); COL9A3: 1564-2012 of L41162 (1196420); BRK: 814-2169 of X78549 (515025).

View larger version (36K): [in this window] [in a new window] [Download PPT slide]   Fig. 3. A, the map position of Sik relative to other markers in The Jackson Laboratory BSS Interspecific Backcross. Only those genes whose human homologues have been mapped are shown. The raw typing data for all of the markers is available on the World Wide Web at http://www.jax.org/resources/documents/cmdata. Distances between markers are given to the left of the chromosome as cM ± SE. B, isochore G + C differences in distal mouse chromosome 2 and human chromosome 20q. Known sequences for the syntenic genes above are analyzed for total G + C content, third codon position G + C content, and o/e (Obs/Exp) CpG ratio for human (H), mouse (M), and the degree to which the human exceeds mouse content (). The percentage of nt sequence identity (with <0.6% gaps) is also indicated (Cons). Note that the GC-rich distal genes, including BRK/Sik, vary in a manner consistent with loss of the most GC-rich isochores in the mouse, but additionally in correlation with map position. The asterisk indicates that mouse Pck1 sequence was assembled from mouse EST fragments and is less reliable. The segments examined are restricted to the coding sequence and usually include all of the coding sequence, but segments of Lama5 and Col9a3 compared use only the 3' sequence because the 5' sequence is unknown.

RNase Protection Assays.
Expression of Sik and BRK was analyzed by RNase protection assay, as described previously (1 , 16) , using [³²P]-CTP-labeled antisense RNA probes. A pBlueScript SK II+ plasmid containing a 205-bp fragment encoding a portion of the Sik catalytic domain (1) was linearized at an XbaI site in the polylinker, and in vitro transcription was performed using T7 polymerase (Promega, Madison, WI). A 198-bp StuI-ApaI fragment of the BRK cDNA was subcloned into pBlueScript SK II-. This plasmid was linearized with HindIII, and in vitro transcription was performed with T7 polymerase. Linearized templates used for in vitro transcription were purified on 5% acrylamide gels. As controls for RNA levels and integrity, RNase protections were also performed with antisense probes for mouse or human cyclophilin (pTRI-cyclophilin-mouse and pTRI-cyclophilin-human; Ambion).

Total RNA from mouse tissues was prepared by homogenization in guanidine thiocyanate solution with 2-mercaptoethanol followed by CsCl gradient centrifugation (17) . Total RNA from human colon tumors and adjacent normal colon tissue was a generous gift from Robert M. Lee and N. O. Davidson (University of Chicago). Twenty µg (mouse) or 10 µg (human) of each total RNA sample or an equal amount of baker’s yeast tRNA was precipitated with ethanol and resuspended in 30 µl of hybridization buffer containing 2 x 10⁵ cpm of probe. The concentration and quality of the RNA were confirmed on stained 4-morpholinepropanesulfonic acid/formaldehyde gels.

Semiquantitative RT-PCR.
The SuperScript Preamplification System (Life Technologies, Inc.) and 2 µg of total RNA were used for synthesis of cDNA. PCR was performed in 20 µl containing 80 ng of cDNA, 50 pmol of each primer, 0.2 mM deoxynucleotide triphosphate mix, 1.2 mM MgCl₂, 20 mM Tris-HCl (pH 8.4), and 50 mM KCl. PCR was done using the following parameters: (a) denaturation, 45 s at 94°C; (b) annealing, 45 s at 67°C; and (c) extension, 1 min at 72°C. For each combination of primers, the kinetics of PCR amplification was studied, and the number of cycles corresponding to the plateau were determined. PCR was performed at an exponential range (29 cycles for BRK; 25 cycles for keratin 8). A 224-bp BRK PCR product was generated using primers Brk-1 (5'- ATCCAGGCCATGAGAAGC-3') and Brk-2 (5'- TGGATGTAATTCTGCGACTCC-3'), corresponding to nt 706–724 and nt 929 to 909 of the Brk sequence. A 110-bp K8 PCR product was generated using primers K8-305 (5'-TTGCCTCCTTCATAGACAAGG-3'), corresponding to nt 305–326, and K8-415 (5'-TGTTGTCCATGTTGCTTCG-3'), corresponding to nt 396–415 of the human K8 gene sequence. PCR products were separated on a 2% agarose gel and stained with ethidium bromide. Bands corresponding to each specific PCR product were quantitated using NIH Image.⁶

Western Blot Analyses.
Total protein was isolated from pinch biopsies or cultured cells. Samples were lysed in radioimmunoprecipitation assay buffer (1 x PBS, 1% NP40, 0.5% sodium deoxycholate, and 0.1% SDS). Twenty µg (tissue) or 30 µg (cell lines) of protein per lane were subjected to electrophoresis through a 10% SDS-polyacrylamide gel and transferred to Immobolin P membranes. Filters were blocked for 1 h in 5% nonfat dry milk in buffer containing 10 nm Tris-HCl (pH 7.5), 500 mM NaCl, and 0.1% Tween 20 and then incubated for 1 h with BRK (C-17) antibody (Santa Cruz Biotechnology), or they were blocked with buffer containing 10 mM Tris-HCl (pH 7.5), 100 mM NaCl, 0.1% Tween 20 and then incubated with ß-antibody for 1 h. (Sigma Chemical Co., St. Louis, MO). The higher NaCl substantially reduced background obtained with the commercially available BRK polyclonal antibody. Subsequently, the membranes were stained with appropriate horseradish peroxidase-conjugated secondary antibodies, and antibody binding was detected using the SuperSignal ULTRA chemiluminescence substrate (Pierce). In control experiments, the immunogenic peptide specifically competed out BRK antibody binding, confirming the specificity of the signal.

In Situ Hybridizations.
BRK mRNA expression in the human intestine was examined using in situ hybridization techniques as described previously (2) . The cRNA probe was prepared from a template consisting of an 884-bp SacI-EcoRI fragment of human BRK cDNA cloned into pBluescript II SK. The in vitro transcription product was labeled with ³⁵S-labeled UTP and hydrolyzed to fragments of an average size of 150 nt in length for better tissue penetration. After hybridization, slides were treated with RNase A for excess probe removal, washed with increasing stringency to 0.1% SSC at 55°C, and dehydrated in graded ethanols diluted with 0.3 M sodium acetate. Sections were coated with autoradiographic emulsion and exposed for 8–11 days at room temperature.

Indirect Immunohistochemistry with Tyramide Amplification.
Paraffin-embedded biopsy samples sectioned at 5–8 µm thick were deparaffinized, hydrated, and preincubated in block buffer [0.1 M Tris-HCl (pH 7.5), 0.15 M NaCl, and 0.05% Tween 20; 1:50 normal goat serum] for 40 min. Sections were then incubated with 0.2 µg/ml BRK antibody (Santa Cruz Biotechnology) in block buffer overnight at 4°C, washed, and incubated with 1:250 biotinylated goat antirabbit antibody (Vector Laboratories) in block buffer for 30–60 min. After washing, the TSA-Indirect Kit (DuPont New England Nuclear) was used according to the manufacturer’s instructions. Briefly, sections were treated with strepavidin-horseradish peroxidase, reacted for 5 min with biotinyl tyramide reagent, visualized with 1:500 FITC-avidin DCS (Vector Laboratories), and mounted with Vectashield mounting medium (Vector Laboratories). For control sections, 4 ng/ng BRK antibody of the peptide from which the BRK antibody was raised (Santa Cruz Biotechnology) were added to block buffer, 10–15 min before use.

	RESULTS

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
The Breast Tumor Kinase BRK Is the Human Orthologue of Mouse Sik.
To isolate the human orthologue of Sik, we screened a normal human small intestine cDNA library (Clontech) with mouse Sik cDNA. From 10⁶ recombinant phage, three positive clones were isolated. These partial cDNA clones shared sequence identity with the nonreceptor tyrosine kinase BRK that was isolated from a human metastatic breast tumor (4) .

Like Sik, BRK is also a 451-amino acid protein with SH2 and SH3 domains and putative regulatory tyrosines at the activation loop and COOH terminus. Unlike members of the SRC family, Sik and BRK each lack consensus myristoylation motifs at the NH₂ terminus. Sik and BRK also have the sequence HRDLAARN in their catalytic domains, in contrast to the HRDLRAAN sequence shared by members of the SRC family. The amino acid sequences of Sik and BRK are aligned in Fig. 1 . Whereas the functional domains of BRK and Sik are conserved, Sik and BRK share only 80% amino acid identity and 83% nt identity.

View larger version (31K): [in this window] [in a new window] [Download PPT slide]   Fig. 1. BRK and Sik protein share an 80% sequence identity. The amino acid sequences of Sik (2) and BRK (4) are aligned, and the differences between the sequences are distributed throughout the different domains. The first circled P (phosphate) corresponds to the phosphorylated tyrosine at the ATP binding site, and the second circled P corresponds to the putative regulatory tyrosine in the COOH-terminal region. The SH3 and SH2 domains of Sik and BRK are marked.

Because of the relatively low level of sequence identity (80%) between Sik and BRK, we performed Southern hybridization experiments to confirm that Sik and BRK are true orthologues. ³²P-labeled BRK and Sik probes were hybridized with restricted mouse and human genomic DNA. Stringent hybridization with probe from the same species indicated the position of bands for each gene. If the probe from the other species recognized a gene of equal or greater homology, an additional set of bands would be visible; however, both the mouse Sik probe and the human BRK probe detect the same fragments in mouse and human genomic DNA as shown in Fig. 2 , confirming that Sik and BRK are the closest homologues of one another.

View larger version (78K): [in this window] [in a new window] [Download PPT slide]   Fig. 2. BRK is the human orthologue of mouse Sik. Mouse (A) and human (B) genomic DNAs were digested with BamHI (Lanes 1), HindIII (Lanes 2), BamHI/HindIII (Lanes 3), and SstI (Lanes 4); electrophoretically separated; transferred to nitrocellulose membranes; and hybridized with Sik and BRK 32P-labeled probes. The Sik and BRK probes hybridize with the same fragments in human and mouse DNA. Because no additional bands appear, we can conclude that no other sequences of equal or greater homology are present in either genome.

The mouse Sik gene is linked to the gene Eef1a2 that encodes translation elongation factor -2. A BAC library constructed from 129/Sv ES cell DNA was screened with primers corresponding to Eef1a2 (25) . Two independent clones were isolated, each containing a 65–70-kb insert. Each was found by sequencing to contain the coding and 3'-UTR sequence of the Sik gene in addition to Eef1a2. One clone also contained all of the 5'-UTR sequence of Sik. The Sik gene must therefore map to the distal end of mouse chromosome 2, within 60 kb of Eef1a2, in a region of conserved synteny with human chromosome 20q13 (Fig. 3) . Because BRK maps to human chromosome 20q13.3 (8) , this provides further evidence that these two genes are orthologous. In wasted mice, the Eef1a2 gene is deleted (25) , but the Sik gene is intact and appropriately expressed.⁷

The coding sequences of BRK and the linked genes EEF1a2 and LAMA5 contain 82–89% G + C in the third codon position, which places them well above the threshold of the H3 isochore (75%), the G + C-richest fraction of DNA that forms 3% of the human genome and contains 28% of human genes (26) . H3 isochores, which are usually over 300 kb in length, are most concentrated in T (telomeric, thermally resistant, or H3+) bands and occur more sparsely in T' (H3*) bands; one of the human genome’s 28 H3+ bands maps to the telomere of chromosome 20 (27 , 28) . Although overall values for G + C% and 5-methylcytosine in human and mouse are nearly identical (24) , the mouse genome lacks the very GC-rich H3 isochore (29 , 30) . Accordingly, the mouse Sik, Eef1a2, and Lama5 genes contain 14–19% less G + C in the third codon position. Interestingly, the tightly linked Col9a3 gene also has 18% less G + C, although its third codon G + C is much lower. It has been estimated that 20% of the CpG islands present in the human have been lost in mouse orthologues, primarily in tissue-specific genes (31) . The case of BRK and Sik suggests that this can occur by effects on the isochore level that increase CpG loss uniformly on a megabase scale. Thus, the conserved synteny of these genes in human and mouse chromosomes near the telomere allows the physical extent and nature of T band changes between the species to be examined directly.

Tissue-specific Expression of Sik in the Mouse.
Sik mRNA expression has only been detected in regenerating epithelia such as that lining the gastrointestinal tract, as well as in the liver and skin. Little or no mRNA expression was detected in the kidney, lung, spleen, testis, uterus, diaphragm, or brain (1 , 2) .⁸ We examined Sik mRNA expression in the mouse small and large intestine (Fig. 4B) by RNase protection. Levels of the Sik protected fragment increase from the duodenum to the ileum, with the ileum having peak levels of Sik mRNA expression.

View larger version (60K): [in this window] [in a new window] [Download PPT slide]   Fig. 4. Tissue-specific expression of Sik in the mouse. A, RNase protection assays were performed to examine Sik expression in the duodenum, jejunum, ileum, and colon. Lane M, marker lane; Lane Pr, undigested probe; Lane t, tRNA sample (negative control). B, to examine the level of active Sik protein in different mouse tissues, Sik was immunoprecipitated as indicated from the brain, spleen, tongue, ileum, liver, and muscle, and in vitro kinase assays were performed. Autophosphorylated Sik protein can be detected only after immunoprecipitation from ileum extract. This band is eliminated by the addition of Sik peptide to the immunoprecipitation reaction (Sik antibody + peptide). C, Sik is not expressed in normal mouse breast tissue. RNase protection assays were performed with total RNA isolated from virgin, pregnant, lactating, and involuting breast tissue, as well as gut (small intestine) and skin.

Sik expression was also examined in the mammary gland. Mammary gland differentiation is regulated hormonally and requires pregnancy for the establishment of terminal differentiation (for a review, see Ref. 32 ). During involution after weaning, a number of morphological and biochemical changes occur. We examined Sik expression in the mammary glands of virgin, pregnant, and lactating mice and at different times after weaning. At no time did we detect expression in the normal mammary gland. In contrast, significant levels of Sik expression were detected in the skin and small intestine (Fig. 4A) . Sik expression was also not detected in the mammary gland at these stages using in situ hybridization and immunohistochemistry (data not shown), ruling out the possibility that Sik expression was induced in a small subset of the cells. We have also not detected Sik expression in the NMuMG normal mouse mammary gland cell line (Ref. 33 ; data not shown).

BRK Expression in Colon Tumor Cell Lines.
BRK expression was examined in the human colon carcinoma tumor cell lines SW480, HT29, T84, and Caco-2. Caco-2 cells, which differentiate spontaneously after becoming confluent, provide a model system for studying enterocyte differentiation. As these cells are maintained in culture, they polarize, form microvilli, and express increasing levels of brush border enzymes, such as sucrase isomaltase (34) . Caco-2 cells are poorly tumorigenic in nude mice when compared with SW480 and HT29 cells (35) . Using RNase protection assays, high levels of BRK mRNA were detected in SW480 and HT29 cells (Fig. 5A) , but low levels were present in Caco-2 and T84 cells. BRK mRNA levels increased 4-fold as Caco-2 cells differentiated, with peak levels appearing at 14 days after plating. This increase in BRK expression levels was detected in different stocks of Caco-2 cells as well as in total and polyadenylated RNAs. Expression of BRK was not detected in the Hep3B liver hepatoma cell line.

View larger version (57K): [in this window] [in a new window] [Download PPT slide]   Fig. 5. BRK expression in colon carcinoma cell lines. A, RNase protection assays were performed with total RNAs isolated from SW480, T84, HT29, and Caco-2 cells, which were derived from adenocarcinomas of the colon, and the Hep3B hepatoma line. SW480 and HT29 cells express high levels of BRK mRNA. Levels of BRK mRNA increase approximately 4-fold during differentiation of the Caco-2 cell line. Results are shown for total and polyadenylated enriched RNAs from two different stocks of Caco-2 cells. Hep3B cells do not express BRK. B, Western blotting was performed with total protein extracts from MCF-7, SW480, HT29, T84, and Caco-2 cells. SW480 and HT-29 cell extracts contain the highest levels of BRK, whereas Caco-2 cells contain too low a level of BRK to be visible in the 10-min exposure at the left. In the 5-h exposure at the right, BRK protein levels can be seen to increase during early differentiation of Caco-2 cells, but the peak protein expression (7 days after plating) does not correspond with the peak mRNA expression (14 day after plating in A). The membrane was stripped and probed with anti-ß-actin antibody as a control (exposure, 2 min).

BRK Is Expressed in the Normal Human Gastrointestinal Tract and in Colon Tumors.
Biopsy samples from esophagus, stomach, duodenum, and colon epithelia were obtained, and total proteins were extracted. The pinch biopsy samples were composed primarily of surface epithelial tissue. Using a rabbit anti-BRK polyclonal antibody, BRK protein expression was detected in all human gastrointestinal tissues that we examined (Fig. 6A) . Significant levels of Sik expression have also been detected in the epithelium of the mouse fetal stomach (2) and adult stomach and esophagus.⁸

View larger version (54K): [in this window] [in a new window] [Download PPT slide]   Fig. 6. BRK is expressed throughout the normal human gastrointestinal tract and in colon tumors. A, Western blot analysis was performed with total human proteins from pinch biopsies from the esophagus, stomach, duodenum, and colon. Identical filters were incubated with BRK antibody (top panel) or with ß-actin antibody (bottom panel) as a control for protein levels. B, RNase protection assays were performed with 10 µg of total RNA from five colon tumor samples and adjacent normal tissue. Increased BRK expression was detected in total RNA from three tumor samples (T1, T2, and T5) when compared to adjacent normal tissue. C, RT-PCR was used to examine BRK and keratin 8 mRNA expression in the five colon tumor samples and adjacent normal tissue. After normalization to the amount of epithelial keratin in each sample, a 2-fold increase in BRK levels was detected in tumors T1 and T5.

We examined BRK expression in the normal human colon and colon tumors using in situ hybridization and immunocytochemistry. BRK mRNA can be detected at the highest levels in the upper crypts in cells that are exiting the cell cycle and undergoing terminal differentiation in the normal colon (Fig. 7A) . These data coincide with the findings obtained for the murine orthologue Sik (2) . Higher levels of hybridization grains were apparent over the disorganized cells of moderately differentiated human colon adenoma (Fig. 7, C and D , open arrow) than in adjacent normal epithelium (closed arrow). A higher magnification of a portion of the tumor is shown in Fig. 7, E and F , which shows variability in the levels of BRK RNA expressed within the tumor.

View larger version (176K): [in this window] [in a new window] [Download PPT slide]   Fig. 7. BRK mRNA is expressed in an epithelial-specific and differentiation-specific manner in normal human colon and at increased levels in a colon tumor. In situ hybridizations were performed with 35S-labeled sense and antisense cRNA probes that correspond to a fragment of the BRK cDNA. Bright-field (A, C, and E) and dark-field (B, D, and F) views of the tissue and emulsion silver grains are shown. In normal colon (A and B), epithelium hybridized strongly and specifically with BRK probe, particularly at and above the cuff region at which colonocytes undergo terminal differentiation (arrow). In colon adenocarcinoma (C and D), BRK signal is present in normal colonic crypts (closed arrow) and transformed tissue (open arrow). At high magnification (E and F), Brk signal over the upper crypt (closed arrow) appears to exceed that of some regions of the tumor (open arrow), but is itself exceeded by the strong signal present in a large portion of the main tumor mass. The sense probe hybridization produced no signal over background (data not shown). Bars, 50 µm.

View larger version (137K): [in this window] [in a new window] [Download PPT slide]   Fig. 8. Immunohistochemical de-tection of BRK expression in normal human colon tissue and archival human colon tumor samples. A, in the normal human colon, BRK protein expression is induced in the upper crypt epithelium (arrows) and is present in the surface epithelium. BRK is also expressed in epithelial cells of three different colon tumors (B, D, E, and F). Specificity is indicated by the lack of signal in the controls in which BRK antibody was preincubated with the synthetic peptide used for immunization (C and G); similar control results were obtained for the samples shown in A and D (data not shown). Arrows in B indicate a transition between high and low levels of BRK in a villus-like region of colon adenocarcinoma, one of several such regions in this tumor; E, two isolated BRK-expressing cells in a monolayer with many transitions in BRK status (this disorganized monolayer represents part of a large adenocarcinoma that does not contain detectable BRK in most regions); F, a transition between sporadic and widespread BRK expression with a granule-specific intracellular distribution within a disorganized colon adenocarcinoma. Bars, 50 µm.

	DISCUSSION

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We isolated BRK encoding cDNA clones from a normal human small intestine cDNA library using a mouse Sik probe. The genes encoding Sik and BRK do not appear to be tightly conserved. In contrast to mouse and human SRC, which share a high degree of sequence identity (99%), mouse Sik and human BRK share only 80% amino acid sequence identity. Because of this relatively low level of homology, we confirmed that Sik and BRK are orthologues of one another by performing a series of Southern blot experiments. We found that radiolabeled probes specific for BRK and Sik recognized an identical simple set of bands in both mouse and human genomic DNA, indicating that no genes with closer homology existed in either genome. In addition, we mapped the Sik gene to the distal portion of mouse chromosome 2, which shows conservation of synteny with human chromosome 20q13.3 where BRK is located.

Because BRK was initially cloned from metastatic breast tumor RNA, we examined its expression during breast development in the mouse to determine whether it plays a role in normal differentiation. We were unable to detect Sik expression at any stage of normal mammary gland development in the mouse. BRK expression in breast tumors and breast tumor cell lines, but not in normal breast tissue, has suggested a role for BRK expression in carcinomas. BRK was found to be expressed at appreciable levels in approximately two-thirds of the breast tumors examined (5) . Overexpression of BRK in the HB4a human mammary cell line mitogenically sensitizes these cells to epidermal growth factor. In addition, overexpression of BRK in these cells resulted in increased growth in soft agar, indicating that BRK overexpression can contribute to a transformed phenotype (40) .

We determined that BRK is expressed in tumor cell lines derived from adenocarcinomas of the colon. Using different methodologies, we also detected moderate increases in BRK RNA and protein expression in primary human colon tumor samples. Whereas the BRK colon tumor data are only of preliminary statistical significance, they consistently favor the notion of a modest increase in BRK in colon tumor tissue, which falls short of the more dramatic induction reported for breast carcinomas. The increase detected in colon tumors may not be related to factors such as gene amplification, which would be expected to yield larger increases. The activity of BRK in colon tumors has not been examined, and it is possible that increases in BRK expression do not reflect increased kinase activity. Mutations of the BRK gene in tumors have not been reported. The sequence of BRK isolated from tumor cells and normal cells appears to be identical thus far (38 , 39) , suggesting that BRK overexpressed in tumor cells is the normal protein.

Several studies suggest that the related SRC family tyrosine kinases participate in the development of colon cancer. SRC tyrosine kinase activity was found to be increased in human colon tumor tissue and in a variety of colon carcinoma cell lines when compared with normal adjacent tissues and normal colonic epithelial cells (41, 42, 43, 44) . SRC activity was found to progressively increase as adenomas become carcinomas, and the highest levels of SRC activity were found in metastatic lesions in the liver (45) . Recently, an activating mutation in SRC codon 531 was identified in 12% of advanced colon tumors examined, providing the first genetic evidence for a role for SRC in colon cancer (46) . A significant increase in the activity of YES has also been observed in colon tumors and in colon carcinoma cell lines (47 , 48) , although no increase in the activities of some other SRC family members such as LCK, FYN, HCK, or FGR was detected (47) .

We found that BRK is present throughout the normal human gastrointestinal tract, in the esophagus, stomach, duodenum, and colon. We localized BRK expression to differentiating epithelial cells in the colon, where the highest levels of protein and mRNA were found in epithelial cells in the middle and upper colonic crypts. We also found that BRK expression increased during the early stages of Caco-2 cell differentiation in vitro. These data support the hypothesis that BRK may play a role in a signal transduction pathway associated with differentiation. In previous studies, we found that mouse Sik is expressed in a differentiation-specific manner in regenerating epithelial linings. Sik was shown to associate with a GAP-binding protein, possibly linking it to the Ras pathway. It will be important to determine the role of this epithelial-specific tyrosine kinase during normal differentiation and to unveil its potential relationship to the development of breast and colon cancers.

	ACKNOWLEDGMENTS

 
We thank Drs. Nicholas O. Davidson and Robert M. Lee for generously sharing tumor RNA samples with us and Doreen Chambers for excellent technical assistance. We also thank Dr. Michael Mihalov for providing archival tumor samples and Drs. Thomas Layden, Allan Halline, and Richard Benya for helpful discussions and comments.

	FOOTNOTES

 
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ Supported by NIH Grant DK44525 and Department of the Army Grant DAMD17-96-1-6175 (to A. L. T.).

² Present address: Gastroenterology Section, Germans Trias i Pujol University Hospital, Autonomous University of Barcelona, Barcelona, Spain.

³ Address: Department of Medicine, University of Edinburgh, Edinburgh, United Kingdom.

⁴ To whom requests for reprints should be addressed, at Department of Genetics, M/C 669, University of Illinois College of Medicine, 900 South Ashland Avenue, Chicago, IL 60607. Phone: (312) 996-7964; Fax: (312) 413-0353; E-mail: atyner{at}uic.edu

⁵ The abbreviations used are: GAP, GTPase-activating protein; UTR, untranslated region; RT-PCR, reverse transcription-PCR; nt, nucleotide; o/e, observed/expected.

⁶ NIH Image is available at http://rsb.info.nih.gov/nih-image/.

⁷ C. A. Abbott, unpublished data.

⁸ M. S. Serfas and A. L. Tyner, unpublished data.

Received 12/31/98; revised 4/19/99; accepted 4/22/99.

	REFERENCES

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 

1. Siyanova E. Y., Serfas M. S., Mazo I. A., Tyner A. L. Tyrosine kinase gene expression in the mouse small intestine. Oncogene, 9: 2053-2057, 1994.[Medline]
2. Vasioukhin V., Serfas M. S., Siyanova E. Y., Polonskaia M., Costigan V. J., Liu B., Thomason A., Tyner A. L. A novel intracellular epithelial cell tyrosine kinase is expressed in the skin and gastrointestinal tract. Oncogene, 10: 349-357, 1995.[Medline]
3. Vasioukhin V., Tyner A. L. A role for the epithelial cell-specific tyrosine kinase Sik during keratinocyte differentiation. Proc. Natl. Acad. Sci. USA, 94: 14477-14482, 1997.[Abstract/Free Full Text]
4. Mitchell P. J., Barker K. T., Martindale J. E., Kamalati T., Lowe P. N., Page M. J., Gusterson B. A., Crompton M. R. Cloning and characterisation of cDNAs encoding a novel non-receptor tyrosine kinase, brk, expressed in human breast tumours. Oncogene, 9: 2383-2390, 1994.[Medline]
5. Barker K. T., Jackson L. E., Crompton M. R. BRK tyrosine kinase expression in a high proportion of human breast carcinomas. Oncogene, 15: 799-805, 1997.[Medline]
6. Lee S. T., Strunk K. M., Spritz R. A. A survey of protein tyrosine kinase mRNAs expressed in normal human melanocytes. Oncogene, 8: 3403-3410, 1993.[Medline]
7. Easty D. J., Mitchell P. J., Patel K., Florenes V. A., Spritz R. A., Bennett D. C. Loss of expression of receptor tyrosine kinase family genes PTK7 and SEK in metastatic melanoma. Int. J. Cancer, 71: 1061-1065, 1997.[Medline]
8. Park S. H., Lee K. H., Kim H., Lee S. T. Assignment of the human PTK6 gene encoding a non-receptor protein tyrosine kinase to 20q13.3 by fluorescence in situ hybridization. Cytogenet. Cell Genet., 77: 271-272, 1997.[Medline]
9. Muleris M., Almeida A., Gerbault-Seureau M., Malfoy B., Dutrillaux B. Identification of amplified DNA sequences in breast cancer and their organization within homogeneously staining regions. Genes Chromosomes Cancer, 14: 155-163, 1995.[Medline]
10. Kallioniemi A., Kallioniemi O. P., Piper J., Tanner M., Stokke T., Chen L., Smith H. S., Pinkel D., Gray J. W., Waldman F. M. Detection and mapping of amplified DNA sequences in breast cancer by comparative genomic hybridization. Proc. Natl. Acad. Sci. USA, 91: 2156-2160, 1994.[Abstract/Free Full Text]
11. Courjal F., Theillet C. Comparative genomic hybridization analysis of breast tumors with predetermined profiles of DNA amplification. Cancer Res., 57: 4368-4377, 1997.[Abstract/Free Full Text]
12. El-Rifai W., Harper J. C., Cummings O. W., Hyytinen E. R., Frierson H. F., Jr., Knuutila S., Powell S. M. Consistent genetic alterations in xenografts of proximal stomach and gastro-esophageal junction adenocarcinomas. Cancer Res., 58: 34-37, 1998.[Abstract/Free Full Text]
13. Schlegel J., Stumm G., Scherthan H., Bocker T., Zirngibl H., Ruschoff J., Hofstadter F. Comparative genomic in situ hybridization of colon carcinomas with replication error. Cancer Res., 55: 6002-6005, 1995.[Abstract/Free Full Text]
14. Sanger F., Nicklen S., Coulsen A. R. DNA sequencing with chain terminating inhibitors. Proc. Natl. Acad. Sci. USA, 74: 5463-5467, 1977.[Abstract/Free Full Text]
15. Rowe L. B., Nadeau J. H., Turner R., Frankel W. N., Letts V. A., Eppig J. T., Ko M. S., Thurston S. J., Birkenmeier E. H. Maps from two interspecific backcross DNA panels available as a community genetic mapping resource. Mamm. Genome, 5: 253-274, 1994.[Medline]
16. Serfas M. S., Tyner A. L. HNF-1 and HNF-1ß expression in mouse intestinal crypts. Am. J. Physiol., 265: G506-G513, 1993.[Abstract/Free Full Text]
17. Chirgwin J. M., Przybyla A. L., MacDonald R. J., Rutter W. J. Isolation of biologically active ribonucleic acid from sources enriched in ribonuclease. Biochemistry, 18: 5294-5299, 1979.[Medline]
18. Quentin Y. A master sequence related to a free left Alu monomer (FLAM) at the origin of the B1 family in rodent genomes. Nucleic Acids Res., 22: 2222-2227, 1994.[Abstract/Free Full Text]
19. Zietkiewicz E., Labuda D. Mosaic evolution of rodent B1 elements. J. Mol. Evol., 42: 66-72, 1996.[Medline]
20. Labuda D., Sinnett D., Richer C., Deragon J. M., Striker G. Evolution of mouse B1 repeats: 7SL RNA folding pattern conserved. J. Mol. Evol., 32: 405-414, 1991.[Medline]
21. Jurka J., Milosavljevic A. Reconstruction and analysis of human Alu genes. J. Mol. Evol., 32: 105-121, 1991.[Medline]
22. Mazzarella R., Schlessinger D. Duplication and distribution of repetitive elements and non-unique regions in the human genome. Gene (Amst.), 205: 29-38, 1997.[Medline]
23. Vidal F., Mougneau E., Glaichenhaus N., Vaigot P., Darmon M., Cuzin F. Coordinated posttranscriptional control of gene expression by modular elements including Alu-like repetitive sequences. Proc. Natl. Acad. Sci. USA, 90: 208-212, 1993.[Abstract/Free Full Text]
24. Jabbari K., Caccio S., Pais de Barros J. P., Desgres J., Bernardi G. Evolutionary changes in CpG and methylation levels in the genome of vertebrates. Gene (Amst.), 205: 109-118, 1997.[Medline]
25. Chambers D. M., Peters J., Abbott C. M. The lethal mutation of the mouse wasted (wst) is a deletion that abolishes expression of a tissue-specific isoform of translation elongation factor 1, encoded by the Eef1a2 gene. Proc. Natl. Acad. Sci. USA, 95: 4463-4468, 1998.[Abstract/Free Full Text]
26. Mouchiroud D., D’Onofrio G., Aissani B., Macaya G., Gautier C., Bernardi G. The distribution of genes in the human genome. Gene (Amst.), 100: 181-187, 1991.[Medline]
27. Saccone S., Caccio S., Kusuda J., Andreozzi L., Bernardi G. Identification of the gene-richest bands in human chromosomes. Gene (Amst.), 174: 85-94, 1996.[Medline]
28. Saccone S., De Sario A., Della Valle G., Bernardi G. The highest gene concentrations in the human genome are in telomeric bands of metaphase chromosomes. Proc. Natl. Acad. Sci. USA, 89: 4913-4917, 1992.[Abstract/Free Full Text]
29. Bernardi G. The isochore organization of the human genome. Annu. Rev. Genet., 23: 637-661, 1989.[Medline]
30. Bernardi G. The isochore organization of the human genome and its evolutionary history: a review. Gene (Amst.), 135: 57-66, 1993.[Medline]
31. Antequera F., Bird A. Number of CpG islands and genes in human and mouse. Proc. Natl. Acad. Sci. USA, 90: 11995-11999, 1993.[Abstract/Free Full Text]
32. Hennighausen L., Robinson G. W. Think globally, act locally: the making of a mouse mammary gland. Genes Dev., 12: 449-455, 1998.[Free Full Text]
33. Hynes N. E., Jaggi R., Kozma S. C., Ball R., Muellener D., Wetherall N. T., Davis B. W., Groner B. New acceptor cell for transfected genomic DNA: oncogene transfer into a mouse mammary epithelial cell line. Mol. Cell. Biol., 5: 268-272, 1985.[Abstract/Free Full Text]
34. Pinto M., Robine-Leon S., Appay M. D., Kedinger M., Triadou N., Dussaulx E. B. L., Simmon-Assmann P., Haffen K., Fogh J., Zweibaum A. Enterocyte-like differentiation and polarization of the human colon carcinoma cell line CaCo-2 in culture. Biol. Cell, 47: 323-330, 1983.
35. de Vries J. E., Dinjens W. N., De Bruyne G. K., Verspaget H. W., van der Linden E. P., de Bruine A. P., Mareel M. M., Bosman F. T., ten Kate J. In vivo and in vitro invasion in relation to phenotypic characteristics of human colorectal carcinoma cells. Br. J. Cancer, 71: 271-277, 1995.[Medline]
36. Koletsky A. J., Harding M. W., Handschumacher R. E. Cyclophilin: distribution and variant properties in normal and neoplastic tissues. J. Immunol., 137: 1054-1059, 1986.[Abstract]
37. Chang T. J., Juan C. C., Yin P. H., Chi C. W., Tsay H. J. Up-regulation of ß-actin, cyclophilin and GAPDH in N1S1 rat hepatoma. Oncol. Rep., 5: 469-471, 1998.[Medline]
38. Mitchell P. J., Barker K. T., Shipley J., Crompton M. R. Characterisation and chromosome mapping of the human nonreceptor tyrosine kinase gene, brk. Oncogene, 15: 1497-1502, 1997.[Medline]
39. Lee H., Kim M., Lee K. H., Kang K. N., Lee S. T. Exon-intron structure of the human PTK6 gene demonstrates that PTK6 constitutes a distinct family of non-receptor tyrosine kinase. Mol. Cells, 8: 401-407, 1998.[Medline]
40. Kamalati T., Jolin H. E., Mitchell P. J., Barker K. T., Jackson L. E., Dean C. J., Page M. J., Gusterson B. A., Crompton M. R. Brk, a breast tumor-derived nonreceptor protein tyrosine kinase sensitizes mammary epithelial cells to epidermal growth factor. J. Biol. Chem., 271: 30956-30963, 1996.[Abstract/Free Full Text]
41. Bolen J. B., Veillette A., Schwartz A. M. Activation of pp60 c-src protein kinase is an early event in colonic carcinogenesis. Proc. Natl. Acad. Sci. USA, 87: 2251-2255, 1987.
42. Cartwright C. A., Kamps M. P., Meisler A. I., Pipas J. M., Eckhart W. pp60 c-src activation in human colon carcinoma. J. Clin. Investig., 83: 2025-2033, 1989.
43. Cartwright C. A., Meisler A. I., Eckhart W. Activation of the pp60c-src protein kinase is an early event in colonic carcinogenesis. Proc. Natl. Acad. Sci. USA, : 558-562, 1990.
44. Cartwright C. A., Coad C. A., Egbert B. M. Elevated c-src tyrosine kinase activity in premalignant epithelia of ulcerative colitis. J. Clin. Investig., 93: 509-515, 1994.
45. Talamonti M. S., Roh M. S., Curley S. A., Gallick G. E. Increase in activity and level of pp60 c-src in progressive stages of human colorectal cancer. J. Clin. Investig., 91: 53-60, 1993.
46. Irby R. B., Mao W., Coppola D., Kang J., Loubeau J. M., Trudeau W., Karl R., Fujita D. J., Jove R., Yeatman T. J. Activating SRC mutation in a subset of advanced human colon cancers. Nat. Genet., 21: 187-190, 1999.[Medline]
47. Park J., Meisler A. I., Cartwright C. A. c-Yes tyrosine kinase activity in human colon carcinoma. Oncogene, 8: 2627-2635, 1993.[Medline]
48. Pena S. V., Melham M. F., Meisler A. I., Cartwright C. A. Elevated c-yes tyrosine kinase activity in premalignant lesions of the colon. Gastroenterology, 108: 117-124, 1995.[Medline]

This article has been cited by other articles:

				C.-H. Shen, H.-Y. Chen, M.-S. Lin, F.-Y. Li, C.-C. Chang, M.-L. Kuo, J. Settleman, and R.-H. Chen Breast Tumor Kinase Phosphorylates p190RhoGAP to Regulate Rho and Ras and Promote Breast Carcinoma Growth, Migration, and Invasion Cancer Res., October 1, 2008; 68(19): 7779 - 7787. [Abstract] [Full Text] [PDF]

				H. J. Newbery, D. H. Loh, J. E. O'Donoghue, V. A. L. Tomlinson, Y.-Y. Chau, J. A. Boyd, J. H. Bergmann, D. Brownstein, and C. M. Abbott Translation Elongation Factor eEF1A2 Is Essential for Post-weaning Survival in Mice J. Biol. Chem., September 28, 2007; 282(39): 28951 - 28959. [Abstract] [Full Text] [PDF]

				F. A. Simmen, R. Xiao, M. C. Velarde, R. D. Nicholson, M. T. Bowman, Y. Fujii-Kuriyama, S. P. Oh, and R. C. M. Simmen Dysregulation of intestinal crypt cell proliferation and villus cell migration in mice lacking Kruppel-like factor 9 Am J Physiol Gastrointest Liver Physiol, June 1, 2007; 292(6): G1757 - G1769. [Abstract] [Full Text] [PDF]

				J. H. Ostrander, A. R. Daniel, K. Lofgren, C. G. Kleer, and C. A. Lange Breast Tumor Kinase (Protein Tyrosine Kinase 6) Regulates Heregulin-Induced Activation of ERK5 and p38 MAP Kinases in Breast Cancer Cells Cancer Res., May 1, 2007; 67(9): 4199 - 4209. [Abstract] [Full Text] [PDF]

				A. Haegebarth, W. Bie, R. Yang, S. E. Crawford, V. Vasioukhin, E. Fuchs, and A. L. Tyner Protein tyrosine kinase 6 negatively regulates growth and promotes enterocyte differentiation in the small intestine. Mol. Cell. Biol., July 1, 2006; 26(13): 4949 - 4957. [Abstract] [Full Text] [PDF]

				M. Kasprzycka, M. Majewski, Z.-J. Wang, A. Ptasznik, M. Wysocka, Q. Zhang, M. Marzec, P. Gimotty, M. R. Crompton, and M. A. Wasik Expression and Oncogenic Role of Brk (PTK6/Sik) Protein Tyrosine Kinase in Lymphocytes Am. J. Pathol., May 1, 2006; 168(5): 1631 - 1641. [Abstract] [Full Text] [PDF]

				H. I. Kim and S.-T. Lee An Intramolecular Interaction between SH2-Kinase Linker and Kinase Domain Is Essential for the Catalytic Activity of Protein-tyrosine Kinase-6 J. Biol. Chem., August 12, 2005; 280(32): 28973 - 28980. [Abstract] [Full Text] [PDF]

				P. Zhang, J. H. Ostrander, E. J. Faivre, A. Olsen, D. Fitzsimmons, and C. A. Lange Regulated Association of Protein Kinase B/Akt with Breast Tumor Kinase J. Biol. Chem., January 21, 2005; 280(3): 1982 - 1991. [Abstract] [Full Text] [PDF]

				D. Brehmer, Z. Greff, K. Godl, S. Blencke, A. Kurtenbach, M. Weber, S. Muller, B. Klebl, M. Cotten, G. Keri, et al. Cellular Targets of Gefitinib Cancer Res., January 15, 2005; 65(2): 379 - 382. [Abstract] [Full Text] [PDF]

D. R. Clayburgh, S. Rosen, E. D. Witkowski, F. Wang, S. Blair, S. Dudek, J. G. N. Garcia, J. C. Alverdy, and J. R.