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A Distinct p53 Protein Isoform Signature Reflects the Onset of Induction Chemotherapy for Acute Myeloid Leukemia

Authors' Affiliations: ¹ Hematology Section, Institute of Medicine, University of Bergen; ² Hematology Section, Department of Internal Medicine, Haukeland University Hospital; ³ The Gade Institute, University of Bergen and Haukeland University Hospital, Bergen, Norway; and ⁴ Department of Surgery and Molecular Oncology, University of Dundee, Dundee, United Kingdom

Requests for reprints: Bjorn Tore Gjertsen, Hematology Section, Institute of Medicine, University of Bergen, N-5021 Bergen, Norway. Phone: 47-55-97-50-00; Fax: 47-55-97-29-50; E-mail: bjorn.gjertsen{at}med.uib.no.

	Abstract

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Purpose: The antioncogene protein product p53 has not been studied previously in cancer patients during in vivo chemotherapy. This study examined the early p53 protein and gene expression during induction chemotherapy in acute myeloid leukemia (AML).

Experimental Design: Leukemic cells were collected from five AML patients during their first 18 hours of induction chemotherapy and examined for p53 protein and gene expression by one- and two-dimensional gel immunoblot and high-density gene expression arrays.

Results: Up-regulation of p53 protein expression was detected in AML patients posttreatment in vivo. One- and two-dimensional gel immunoblots showed two main forms of p53, denominated p53 and p53, both recognized by various NH₂-terminal directed antibodies. As a response to treatment, we detected rapid accumulation of p53, with significantly altered protein expression levels already after 2 hours. The accumulation of p53 was accompanied by increased transcription of putative p53 target genes and subsequent cytopenia in the patients.

Conclusion: Up-regulation of the p53 protein and target genes seems to be a prominent feature in induction chemotherapy of AML. The rapid shift from a shorter p53 protein form () toward the full-length protein () underscores the complexity of p53 protein modulation in patients undergoing chemotherapy.

The p53 protein is a sequence-specific transcription factor that can halt progression through the cell cycle or initiate apoptosis on activation by genotoxic stimuli (11). In contrast to other malignancies, where as many as 70% of cases may comprise mutations in TP53 (12), >90% of AML cases have the wild-type gene (13, 14). Development of AML is a result of combined genetic defects, often including constitutive kinase activation together with alterations of transcription factors (15, 16). Gene expression profiling has shown varying kinase and phosphatase expression (17), resulting in altered responsiveness in signaling pathways (18). This may be a possible mechanism for AML blast survival even in the presence of wild-type p53.

The p53 protein is regulated by multiple post-translational modifications in response to chemotherapy as well as other cellular stress inducers (19). Post-translational modifications will contribute to p53 stabilization and accumulation leading to nuclear localization of the protein and specific gene transactivation (19). As many as 1,500 genes have been reported to respond to p53 activation (20) directly or indirectly, including the extensively studied genes p21/cyclin-dependent kinase inhibitor 1A (21), BAX (22), MDM2 (23), and GADD45 (24).

Major variants of the p53 protein may be formed through alternative splicing of mRNA or protein cleavage. To date, the human p53 gene has been reported to encode for 10 isoforms through variously spliced mRNA (25, 26). These are the full-length proteins, three NH₂-terminally truncated isoforms translated from an alternative point of initiation at codon 40 or, by alternative splicing of intron 2 (25, 27, 28), two COOH-terminally truncated isoforms produced by alternative splicing of intron 9 (25, 29), three isoforms produced from an internal promoter in intron 4 (25), and one isoform produced by alternative splicing within exons 7 to 9 (26). In addition, truncated p53 protein products are known produced as a result of protease action most likely through an autoproteolysis mechanism (30, 31). Based on these observations, one would expect the presence of multiple isoforms of p53 protein that could disclose nuances in the cellular response in vivo.

We explored p53 protein modulation in vivo within the first 18 hours after start of chemotherapy. The p53 response was analyzed using information dense methodology like two-dimensional p53 protein analysis and gene arrays with high number of probes (32). A panel of NH₂-terminally directed p53 antibodies showed a dynamic protein response with a shift in p53 isoform distribution and accumulation of the full-length protein. This effect on p53 protein expression was accompanied by putative p53 target gene activation as a response to in vivo chemotherapy in primary AML.

	Materials and Methods

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Patients. The study was approved by the local ethics committee and samples were collected after informed consent. We collected peripheral blood AML blasts from five consecutive patients during chemotherapy by antecubital vein puncture. The patients were treated with i.v. infusion of idarubicine (12 mg/m² during 30 minutes on days 1-3) and cytarabine (190 mg/m² daily as a continuous infusion days 1-7) through a central venous catheter. The clinical and biological characteristics of the patients are presented in Table 1 . Analysis of 20 AML patients showed that the p53 protein pattern shown in the present study was associated with wild-type TP53.⁵

Sample preparation for protein and gene expression analysis. Material for protein analysis was collected as described previously in detail (33, 34). Briefly, cells were washed in NaCl (9 mg/mL) and then lysed in 7% TCA. Protein precipitate was then washed in 5% TCA and water saturated ether to remove salts. The protein pellet was suspended in sample buffer for two-dimensional gel electrophoresis (7 mol/L urea, 2 mol/L thiourea, 100 mmol/L DTT, 1.5% ampholyte 3-10, 0.5% ampholyte 5-6, 0.5% 3-[(3-cholamidopropyl)-dimethylammonio]-1-propane sulfonate). RNA was isolated from AML blasts as described previously (17). Aminoallyl-UTP (Ambion, Cambridgeshire, United Kingdom) was incorporated into cRNA followed by cross-coupling of Cy5 and Cy3 with reactive Cy-NHS compounds (Amersham Biosciences AB, Uppsala, Sweden) to generate fluorochrome-labeled targets for DNA microarray analysis.

Gene expression analysis. The Agilent Human Whole Genome Oligonucleotide Microarray (44K; Agilent Technologies, Inc., Palo Alto, CA) was used for gene expression analysis of patients 1, 4, and 5, and the Human 1 cDNA Microarray (Agilent Technologies) containing 12,814 cDNA clones was used for validation purposes (17). The procedure was done according to the manufacturer's protocols, except for a more stringent wash (0.1 x SSC at 35°C for 10 minutes for the oligonucleotide array). The oligonucleotide microarrays were scanned and features were automatically extracted, recorded, and analyzed using the Agilent Microarray Scanner Bundle. Normalization, flooring, or filtration of data was done according to previously described in-house bioinformatic procedures (17, 35). Rank product analysis (36) was used to detect differentially expressed genes in the oligonucleotide microarray experiments. The data were formatted in a J-Express file suitable for additional data mining.⁶ Selected genes and samples were clustered by hierarchical clustering using average linkage and Pearson correlation as similarity metrics.

For further confirmation of Array data, mRNA level of p21, BAX, PUMA, GADD45, PCNA, and MDM2 was analyzed using Taqman low-density arrays (LDA), 384-well customizable microfluidic cards for real-time PCR (Applied Biosystems, Foster City, CA). Each LDA card was configured for genes in duplicates, including Celera gene ID. Hexamer-primed single-stranded cDNA corresponding to 5 ng AML blast total RNA was diluted in Taqman universal buffer (Applied Biosystems) and added to each loading well. The samples were distributed to the microwells by centrifugation for 1 minutes at 343 x g. The cards were sealed and placed in the ABI 7900 Sequence Detection System using the following cycling variables: 2 minutes at 50°C, 10 minutes at 95°C, and 40 alternate cycles of 15 seconds at 95°C and 60 seconds at 60°C. LDA analysis used GAPDH as normalizer and one sample as calibrator. GAPDH was used for normalization of cDNA microarray values. The SDS2.2 software was used for qualitative analysis and data were exported to Excel spreadsheet (Microsoft, Inc., Seattle, WA) for further exploration and visualization. The correlation coefficients between Array and LDA gene expression values were calculated using XL Statistical Correlation Analysis.

Detection of p53 isoform mRNA expression was done as described previously by Bourdon et al. (25).

Gel electrophoresis and immunoblotting. Protein separation was done by SDS-PAGE following standard procedures. Two-dimensional gel electrophoresis was done using 7-cm pH 3 to 10 (Zoom Strip, Invitrogen Corp., Carlsbad, CA) isoelectric focusing gel strips following the manufacturer's instructions. The focusing strips were incubated with sample rehydration buffer (8 mol/L urea, 1% 3-[(3-cholamidopropyl)-dimethylammonio]-1-propane sulfonate, 20 mmol/L DTT, 1.5% ampholyte 3-10, 0.5% ampholyte 5-6, traces of bromphenol blue) overnight at room temperature to rehydrate the strips. Protein was added directly to the rehydration buffer. Isoelectric focusing was done at 200 V for 40 minutes, 450 V for 30 minutes, 750 V for 30 minutes, and 2,000 V for 60 minutes. Following isoelectric focusing, the strips were either stored at –80°C until further use or equilibrated directly for 15 minutes in LDS sample buffer (Invitrogen) containing 100 mmol/L DTT and then 15 minutes in LDS sample buffer containing 125 mmol/L iodacetamide. For the second dimension, the Zoom strip was aligned in a 0.5% agarose solution added into the isoelectric focusing well of a NuPAGE Novex 4% to 12% Bis-Tris Zoom Gel (Invitrogen). Electrophoresis was done at 200 V for 60 minutes, after which the proteins were transferred to polyvinylidene fluoride membrane by standard electroblotting.

The p53 protein was detected using Bp53-12 monoclonal antibody, recognizing a NH₂-terminal epitope of p53 (epitope mapping amino acids 20-25). Bp53-12 visualized p53 identical to the antibody DO-1 (epitope mapping amino acids 21-25) and Ab-2/PAb1801 in two-dimensional immunoblot (data not shown). p63 protein was detected using primary D-9 antibody, BAX protein was detected using primary 2D2 antibody (Santa Cruz Biotechnology, Santa Cruz, CA), and p21 protein was detected using primary SX118 antibody (BD Biosciences, CA). Actin was detected using primary AC-15 antibody from Abcam (Cambridge, United Kingdom). Secondary horseradish peroxidase–conjugated mouse antibody (Jackson ImmunoResearch, West Grove, PA) was visualized using the SuperSignal West Pico or SuperSignal West Femto Chemoluminescent Substrate (Pierce Biotechnology, Inc., Rockford, IL). The immunoblots were imaged using a Kodak Image Station 2000R (Eastman Kodak Co., Lake Avenue, Rochester, NY), and spots were quantified using the Kodak analysis software. Data were exported to Excel spreadsheet, and a Student's two-tailed t test was used for statistics of the ratio between p53 and p53.

	Results

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p53 and gene expression in human AML cells during in vivo exposure to chemotherapy. In cell protein extract from five AML patients, we found a significant up-regulation of p53 protein in response to induction chemotherapy (Fig. 1A ). Interestingly, p53 protein was present in two isoforms before treatment induction. Only the higher molecular form was up-regulated in response to chemotherapy, whereas the lower molecular form seemed to be down-regulated (Fig. 1A). To determine whether this p53 response lead to the activation of p53-targeted genes, we randomly selected three patients (Table 1, patients 1, 4, and 5) for gene expression analysis (Fig. 1B). mRNA isolated from AML cells before and after 4 hours of chemotherapy was analyzed by Agilent Human Whole Genome Oligonucleotide Microarray and Taqman LDA (Fig. 1B), and the 10 most up-regulated mRNA signals were all putative p53-inducible genes: p53CSV/p53-inducible cell survival factor (37), BAX/BCL2-associated X protein variant ß (22), SES2/hypoxia-induced gene 95 (38, 39), MDM2 (40), GADD45A/growth arrest and DNA damage inducible (24), FDXR/ferridoxin reductase variant 2 (41), BBC3/PUMA/BCL2-binding component 3 (42), TP53INP1/p53-inducible nuclear protein 1 (43), CDKN1A/cyclin-dependent kinase inhibitor 1A (p21; refs. 21, 44), and SESN1/p53-regulated PA26 nuclear protein (45). The increased expression of p53-induced genes was reproduced by mRNA expression analysis of BAX, MDM2, PUMA, GADD45, p21, and PCNA using cDNA microarray (Fig. 1B). The correlation coefficient values in the mRNA expression analysis were 0.95 for BAX, 0.98 for MDM2e, 0.91 for PUMA, 0.92 for GADD45A, 0.86 for p21, and 0.72 for PCNA. For each of the genes, we calculated the fold change (mean value) for Array and LDA gene expression 4 hours after chemotherapy induction. BAX mRNA expression 4 hours following induction was increased 1.7-fold according to Array () and 2.0 times according to LDA () values. The average fold changes 4 hours following induction were 2.1 () and 2.4 () for MDM2e, 3.1 () and 3.7 () for PUMA, 3.9 () and 4.1 () for GADD45A, 4.6 () and 5.2 () for p21, 2.5 () and 2.4 () for PCNA. The false discovery rate of the presented genes varied from <0.05% to 0.1%, and the correlation between the gene expression data obtained from oligonucleotide microarray and cDNA microarray analysis ranged between 85% and 97%. The patients analyzed by microarrays were also investigated by immunoblotting to see whether the results could be confirmed on protein level. Patients 1, 4, and 5 were tested before (–0.5 hour) and after (4 and 18 hours) chemotherapy and all three patients showed induction of p53 protein and the p53-targeted proteins p21 and BAX (Fig. 1C). Taken together, our protein and gene expression analysis in AML cells from patients undergoing chemotherapy suggest that p53 is functional and causes appropriate induction of p53-regulated genes (Fig. 1).

View larger version (30K): [in this window] [in a new window]   Fig. 1. p53 response in de novo AML patients treated with standard chemotherapy. A, a significant p53 protein response after chemotherapy induction with daunorubicine and cytarabine was detected in five AML patients treated in vivo (see Table 1). Cells were collected as described in Materials and Methods before start of induction and at three different time points. The p53 signal was quantified (A, right) and the induction of p53 was found to be significant (P < 0.05). B, relative mRNA abundance in patients 1, 4, and 5 was determined by Agilent 44K DNA Oligonucleotide Microarray () and Taqman quantitative PCR LDA () as described in Materials and Methods. The hierarchical cluster analysis (B, left) shows the 10 highest ranked p53-inducible genes activated by in vivo chemotherapy examined in patients 1, 4, and 5 by oligonucleotide microarray. The heat diagram illustrates changes in mRNA expression in AML blasts from the three patients before treatment and 4 hours after induction chemotherapy. False discovery rates for the 10 genes in the dendrogram were 0.0% to 0.1%, and Ps ranged from 3.9 x 10–11 to 4.1 x 10–8. The relative mRNA abundance measured by microarray and LDA was compared (B, right) in AML blasts before induction therapy (green) and 4 hours after induction (red). The correlation coefficients (CF) between microarray and LDA gene expression values were between 0.72 and 0.98. C, patients 1, 4, and 5 were also subject to protein analysis using standard immunoblotting of p53, p21/CDKN1A, and BAX.

View larger version (40K): [in this window] [in a new window]   Fig. 2. Mapping of the p53 protein by two-dimensional gel electrophoresis and immunoblot and expression of mRNA splice forms. A, our analysis facilitated mapping of total p53 in AML cells detected by antibody Bp53-12, identifying putative p63 (circled top spot), a nonidentified putative p53 cleavage product or short form (bottom dotted spot), and a spot group corresponding to full-length p53 (top dotted spot). B, mRNA of p53 isoforms with intact NH2 terminus (p53, p53ß, and p53) were detected as described previously (25). All three isoforms were detected in patients 1, 4, and 5. C, reproducibility of two-dimensional immunoblot was tested by examining three healthy donors of peripheral blood mononuclear cells (PBMC) in three separate runs of two-dimensional immunoblot, examining total p63 (D-9) and p53 (Bp53-12). Note that the putative p63 is detected by both Bp53-12 and D-9. The estimation of molecular weight (kDa) and isoelectric point (pI) of different p53 family members is described in Materials and Methods.

Modulation of p53 protein patterns by chemotherapy. For examination of p53 modulation after chemotherapy, AML cells derived from five patients sampled in vivo was analyzed using two-dimensional immunoblot. After only 4 hours of treatment, we observed a marked increase in p53 and the p53/p53 ratio (Fig. 3 ). In untreated cells, the ratio usually is p53 > p53, but after cell stress this balance was disturbed and a shift toward p53 was observed. The increase in p53 most likely reflects stabilization of the wild-type, full-length p53 protein. Later during treatment, the increase in p53 was halted possibly through HDM2 feedback down-regulation of p53 (46).

View larger version (44K): [in this window] [in a new window]   Fig. 3. p53 isoform modulation during chemotherapy in vivo. AML cells from patients treated with chemotherapy in vivo were analyzed by two-dimensional immunoblot. Note the shift in p53 from the p53 toward the full-length p53 protein. Control cells were collected 0.5 hours before start of treatment (–0.5 hour). Right, changes in p53/p53 protein ratio in arbitrary units. Representative for two to three independent immunoblots.

	Discussion

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In our analysis of p53 protein in cell samples collected from patients undergoing chemotherapy, we observed a p53 protein induction as would be expected from previous in vitro studies (ref. 47; Fig. 1A). Up-regulation of putative p53 target genes was also observed after chemotherapy (Fig. 1B) and up-regulation of two of these was also verified on the protein level (Fig. 1C). During AML induction, therapy apoptosis was not seen in the peripheral circulation up to 18 hours,⁷ and previous studies have only been able to detect apoptotic AML cells in bone marrow after 24 to 48 hours (48, 49). At the same time, cytopenia developed within 3 to 6 days in our patients (Table 1) with significant decline in peripheral leukemic cells during the first 18 hours. The lack of apoptotic cells in the circulation during induction chemotherapy is probably due to the organism's high capacity of apoptotic cell eradication from peripheral blood by the spleen and liver (50). We therefore suggest that the gene induction observed in this study represents an early chemotherapy-induced event and exhibits the importance of p53-inducible genes in vivo. The majority of the most intensely induced genes (e.g., BAX, PUMA, and TP53INP1) are reported to induce apoptosis if their expression is enforced one by one in vitro (22, 42, 51). On the other hand, p53-inducible cell survival factor (p53CSV) and HDM2 are known to protect against cell death (37, 40), suggesting that this p53 transcriptional induction comprises genes that may improve the efficiency of therapy if targeted.

The p53 protein is extensively regulated post-translationally by phosphorylation, acetylation, sumoylation, neddylation, and ubiquitination (11). Many signaling enzymes known to modify p53 are themselves mutated in cancers, thereby mimicking disease with p53 mutation (52). One of the enzymes of particular interest over the recent years has been Chk2, which has been reported to be mutated in a Li-Fraumeni syndrome family with normal p53 (53). As p53 mutations are rare in AML, kinase or phosphatase mutations may contribute to the AML pathogenesis and be a contributing factor causing incomplete remission. In this study, we used a p53 antibody directed toward the extreme NH₂ terminus of p53 (amino acids 20-25), a region that contains phosphorylation sites modified by Chk2 as well as other cell stress-related kinases (19, 54). The p53 protein isoform distribution could reflect altered expression and/or activity of these kinases in AML, suggestive of a study of the p53 protein in a more extensive AML material. In our study, the two-dimensional immunoblot methodology failed to map the distribution of selected phosphorylated residues in p53 isoforms in resting cells (data not shown). However, it has been shown previously that most of the p53 forms visualized on a two-dimensional map are phosphorylated (55), and future efforts are planned to elucidate the nature of post-translational modifications behind the p53 isoform map.

The known p53 isoforms have been found to possess different functions. Bourdon et al. recently reported that p53 isoforms are expressed in normal human tissue in a tissue-dependent manner (25). They also report differential binding of these isoforms to p53-responsive promoters and alternate apoptotic responses. Detection of a shift toward full-length p53 accompanied by p53 target gene induction in our material suggests that the full-length isoform is the most important isoform in the p53 response to cell stress in AML. The second main isoform found in AML, p53, resembles p53ß and p53 isoforms (25) in size (45 kDa) and pI (5.5; theoretical pI calculated using the Expasy protparam tool⁸). An antibody specific for the p53ß isoform (KJC8; ref. 25) did not, however, reveal any signal resembling p53. The p53 isoform reported by Rohaly et al. (26) is also similar to the p53 found in our material in size and pI. Further experiments are, however, needed to elucidate the exact nature of the p53 isoform.

This work shows that the rapid in vivo activation of the p53 network in response to induction chemotherapy in AML is an important event in leukemic cell debulkment. The complex regulation of the p53 protein during in vivo chemotherapy underscores the feasibility for further characterization of the p53 network in AML.

	Acknowledgments

 
We thank Hua My Hoang, Siv Lise Bedringaas, and Stein-Erik Gullaksen for expert technical assistance.

	Footnotes

 
Grant support: Norwegian Research Council Functional Genomics Program grant 151859 and Norwegian Cancer Society, Kreftforeningen (N. Anensen and B.T. Gjertsen), Norwegian Cancer Society (O. Bruserud), and Helse Bergen and Haukeland University Hospital Research Found (A.M. Oyan and K.H. Kalland).

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.

⁵ N. Anensen and B.T. Gjertsen, submitted for publication.

⁶ http://www.molmine.com/.

⁷ B.T. Gjertsen, unpublished data.

⁸ http://ca.expasy.org/tools/protparam.html.

Received 9/ 9/05; revised 3/20/06; accepted 4/25/06.

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