Quantitative analysis of FJ 194940.1 gene expression in colon cancer and its association with clinicopathological parameters

Malwina Bartczak-Tomczyk; Aleksandra Sałagacka; Marek Mirowski; Agnieszka Jeleń; Ewa Balcerczak

doi:10.5114/wo.2013.33773

. 2013 Mar 15;17(1):45–50. doi: 10.5114/wo.2013.33773

Quantitative analysis of FJ 194940.1 gene expression in colon cancer and its association with clinicopathological parameters

Malwina Bartczak-Tomczyk ¹, Aleksandra Sałagacka ¹, Marek Mirowski ¹, Agnieszka Jeleń ¹, Ewa Balcerczak ^1,^✉

PMCID: PMC3685339 PMID: 23788961

Abstract

Aim of the study

The FJ 194940.1 gene is located on chromosome 1 and consists of 6 exons and 5 introns. The gene undergoes alternative splicing and its isoforms appear during cancer development. Evidence suggests that expression of FJ 194940.1 splice variants relate to colorectal cancer progression. This paper discusses the quantitative analysis of the exon V expression level of FJ 194940.1 in colon cancer. The aim of the study is to carry out quantitative analysis by real-time PCR in a series of 102 colon cancer samples that had previously shown presence of exon V expression. To compare the exon V expression level with certain histological parameters and clinical staging of the neoplasm in order to assess its potential role as a prognostic factor in colon cancer.

Material and methods

Tissue specimens of colorectal cancer were obtained from the Oncological Centre of Lodz, Poland.Total RNA isolation was performed in accordance with the protocol enclosed in the Total RNA Prep Plus Minicolumn Kit (A&A Biotechnology, Poland). Reverse Transcriptase-PCR reaction was carried out using Enhanced Avian HSRT-PCR Kit, Sigma, according to the manufacturer's protocol.. Presence of cDNA in each sample was checked by PCR amplification of β-actin. Only samples showing the PCR product of this housekeeping gene were included in further tests. The amount of FJ 194940.1 transcript containing exon V was analysed by means of real-time PCR.

Results

Exon V expression level is not significantly related to any clinicopathological features in colon cancer. However, there was a tendency towards a lower exon V expression level in a group of cases where vessel invasion was present (p = 0.0697). Additionally, the risk of death in patients with a low exon V expression level was more than two times higher when compared to patients with a high exon V expression level.

Conclusions

FJ 194940.1 gene expression correlates with cancer progression independently of analysed clinicopathological parameters.

Keywords: FJ 194940.1, expression, alternative splicing, transcript, colon cancer

Introduction

Colon cancer is a very serious clinical problem. It is the second most frequent cause of cancer mortality in the world's more developed countries. Over the past 15 years, researchers have submitted a lot of evidence to show that colorectal cancer (CRC) is a progressive genetic disease [1]. It is now clear that neoplasm development is a complex multistep process. Multiple molecular pathways exist in colorectal tumourgenesis in addition to the classic suppressor and mutator mechanisms [2]. Despite the wealth of knowledge that exists regarding the genetic background of this disease, there is still a need to look for some missing points in the development of this tumour.

The characterisation of splicing deregulation in cancer may lead to greater comprehension of malignant transformation, especially as specific alterations in splicing patterns exist in cancer-associated genes. Many of these changes may play a functional role in transformation, motion and metastasis of tumour cells [3, 4]. Alternative splicing variants of those genes may have prognostic or predictive values that could facilitate diagnostic and/or treatment procedures. Consequently, experimental research focuses on splice variants appearing during cancerogenesis, which could potentially become new molecular markers [5]. Abnormal splicing of several genes has been observed in tumours of colorectal origin, e.g. CD44 [6, 7], MUC2 [8], SRF [9], NCAM [10], MLH, MSH [11] and members of the Wnt pathway [12]. There is evidence that FJ 194940.1 gene variants play an important role in colon tumourigenesis [13].

The FJ 194940.1 gene is located on chromosome 1, region 224792167-224794166. In normal human tissues, this chromosome region is expressed as the AK055856 transcript only in the kidney. Probably during cancerogenesis, integration of an additional copy of rv_001141 changes this transcription region. The new transcript has 921 bp and encodes a protein that contains an integrase core domain similar to the human protein EAW69787. Genomic DNA of the new transcript spans 3518 bp and consists of five exons and four introns [14].

Studies have shown that the FJ 194940.1 gene may be a potential molecular marker of cancer development and progression [15–17]. Some of these indicated that the expression of elements of the FJ 194940.1 gene is associated with clinical stages of colon cancer. Expression of the whole exon V of FJ 194940.1 as well as fragments of exon IV and VI was found at advanced stages of cancer development [18]. This observation was further confirmed by quantitative analysis in the same colon cancer cases. A high expression level of this FJ 194940.1 transcript fragment was found in patients with metastases to lymph nodes and distant metastases, and in cases with vessel invasion and absence of lymphocytes in tumour tissue. The level of expression was associated with shorter survival time [16]. Interestingly, the expression of those elements was not regular [18].

A forward preliminary assay has taken into consideration the whole transcript of the FJ 194940.1 gene. This report stated that FJ 194940.1 undergoes alternative splicing. Exon V was irregularly observed in 30 investigated colon cancer cases but its expression was not significantly connected with any clinicopathological features [14].

Results obtained by Bartczak et al. [13] have confirmed that FJ 194940.1 undergoes alternative splicing. Expressions of exons and exon-exon junctions were not associated with any clinicopathological features in colon cancer. On the other hand, exon V, the object of the present study, was an element of the part B transcript (comprising exon IV, V as well as III/IV and IV/V exon-exon junction). The presence of part B expression was connected with cases of low-grade malignancy, which correlated with better prognosis for patients [13]. Importantly, the expression of exon V was found in all of the investigated samples [13].

The discrepancies described regarding the potential prognostic value of FJ 194940.1 gene expression in colon cancer, as well as the precursory character of the mentioned study, indicate the need for a more searching investigation.

The study presented here is a follow-up to the Bartczak et al. experiment [13], where in exon V expression was detected in all examined samples. Additionally, this exon is a part of the FJ 194940.1 transcript fragment that was studied by Balcerczak E. et al. in 2003 [18] and Balcerczak M. et al. in 2007 [16]. The aim of this presented study was to investigate the exon V FJ 194940.1 gene expression level, quantified by real-time PCR, in a series of 102 colon cancer cases, and evaluate its utility as a prognostic marker in colon cancer patients.

Material and methods

Materials

Tissue specimens of colorectal cancer were obtained from the Oncological Centre of Lodz, Poland. CRC was diagnosed by histopathological examination using established clinical criteria (TNM classification by Jass with latest revision Cancer Staging Manual by AJCC, 1997) at the Department of Pathology, Medical University of Lodz, Poland. Tissue samples from 102 patients were frozen in liquid nitrogen immediately after surgery and stored at –80°C until further examination. The characteristics of the examined population are shown in Table 1.

Table 1.

Comparison of FJ 194940.1 exon V expression level with clinicopathological parameters

Feature		n	Median	Minimum	Maximum	Lower quartile	Upper quartile	p value
Gender	female	44	11.21	0.10	1831.97	3.05	42.59	0.2955
Gender	male	35	19.17	0.05	329.69	7.34	42.66	0.2955
Family history	negative	69	16.83	0.10	1831.97	9.04	83.99	0.9003
Family history	positive	10	17.87	0.38	149.63	4.07	30.21	0.9003
Tumour location	rectum	30	13.29	0.16	1832.97	5.22	40.78	0.9672
Tumour location	colon	48	16.70	0.05	1699.60	2.87	48.53	0.9672
Histological type	tubular	69	16.83	0.05	1831.97	4.01	44.40	0.5905
Histological type	mucinous	10	11.35	2.73	105.44	7.68	19.17	0.5905
Histological grade	G1 or G2	57	16.83	0.10	1831.97	5.63	55.32	0.2281
Histological grade	G3	21	12.66	0.05	1699.60	2.81	25.49	0.2281
Invasion of the intestinal wall	T1 or T2	21	16.58	0.10	1831.97	6.81	35.99	0.9823
Invasion of the intestinal wall	T3 or T4	58	16.03	0.05	1699.60	4.01	44.40	0.9823
Node involvement	N0	41	16.58	0.10	1831.97	6.81	42.66	0.7095
Node involvement	pN1 or pN2	34	17.04	0.05	1699.60	4.01	44.40	0.7095
Distant metastasis	M0	61	16.83	0.05	1831.97	5.63	42.66	0.2848
Distant metastasis	M1	18	8.06	0.16	1699.60	2.16	39.57	0.2848
pTNM stage	I or II	40	15.90	0.10	1831.97	6.22	39.32	0.7611
pTNM stage	III or IV	39	16.83	0.05	1699.60	2.81	44.40	0.7611
Lymphocytic infiltration	absent	43	9.47	0.16	1831.97	3.17	55.32	0.4245
Lymphocytic infiltration	present	35	18.14	0.05	1699.60	5.04	42.44	0.4245
Vessel invasion	absent	28	26.69	0.55	1831.97	9.00	60.59	0.0697
Vessel invasion	present	51	12.66	0.05	1699.60	2.94	40.78	0.0697

Open in a new tab

All experiments were carried out with local ethical committee approval (No. RNN/214/00) and patients’ informed consent.

RNA isolation

Total RNA isolation was performed in accordance with the protocol enclosed in the Total RNA Prep Plus Minicolumn Kit (A&A Biotechnology, Poland). The method is based on RNA isolation methodology developed earlier by Chomczynski and Sacchi, 1987 [20]. RNA concentration was determined spectrophotometrically. The isolated RNA had an A260/280 ratio of 1.6–1.8. Purified RNA samples were stored at –80°C.

cDNA synthesis

RT-PCR reaction was carried out using Enhanced Avian HS RT-PCR Kit, Sigma, according to the manufacturer's protocol. The cDNA was used immediately or stored at –20°C. Presence of cDNA in each sample was checked by PCR amplification of β-actin. Only samples showing the PCR product of this housekeeping gene were included in further tests.

Real-time PCR

The amount of FJ 194940.1 transcript containing exon V was analysed by means of real-time PCR.

Amplification reactions were performed using Rotor-Gene 6000 (Corbet) and SYBR Green Jump Start Tag ReadyMix^TM (Sigma) according to the manufacturer's instructions.

The primer set CTCTCTTGCTGAAATGCTGG (forward) and GGCCCAGGCTTTAAACTATA (reverse) and reaction conditions used in the assay were described earlier [14]. The 25 µl reactions consisted of 12.5 µl of JumpStart Taq ReadyMix, 0.5 µl of forward primer (final concentration 0.28 µl), 0.5 µl of reverse primer (final concentration 0.28 µl), 1.5 µl of magnesium chloride (final concentration 3 µl), and 2.5 µl of temple cDNA or sterile water. The thermal cycling conditions were 7 minutes at 95°C, followed by 40 cycles of 60 seconds at 97°C, 60 seconds at 60°C, and 60 seconds at 72°C. Experiments were performed in duplicate to ensure reproducibility of the technique. At the end of each reaction, the threshold was manually set at the level reflecting the best kinetic PCR parameters, the same for all analysed samples. Ct was determined and melting curves were acquired and analysed.

As a reference, the expression of the b-actin gene was quantified for each sample using the 5’-GTGGGGCGCCCCAGGCACCA-3’ (forward), 5’-CTCCTTAATGTCACGCACGATTTC-3’ (reverse) primer set. The reactions for FJ 194940.1 exon V and β-actin were carried out in separate tubes. The 2^–ΔΔ method invented by Livak and Schmittgen [20] was used to calculate relative changes in gene expression determined from real-time quantitative PCR experiments. Real-time PCR assay has a 100% amplification efficiency for both genes and was therefore used in the 2(ΔΔC(T)) method.

Statistical analysis

STATISTICA 9.1 (StatSoft, Inc., 2010) was used for statistical analyses. The collected quantitative data were tested to check for conformity with a normal distribution on the basis of the Shapiro-Wilk test. Due to a lack of conformity in distributions with normal distribution in every subgroup of patients compared, the statistical analysis of the obtained results employed the nonparametric Mann-Whitney U test.

Dependences between clinicopathological characteristics, FJ 194940.1 exon V expression levels and overall survival in the entire population of 79 patients were estimated using the Kaplan-Meier estimator (univariate analysis). Overall survival was determined as the interval between surgery and death. Median overall survival time was 65 months (minimum 1 month, maximum 110 months). The log-rank test was used to test for differences in time-to-death distribution.

A Cox proportional hazard regression model (multivariate analysis) was created to identify the independent prognostic factors. A p-value < 0.05 was assumed as significant in all conducted tests.

Results

Expression analysis was successful in 87 out of 102 cases of colorectal carcinomas taken for analysis. In 15 of the examined samples, no PCR product was obtained for the housekeeping gene, despite RNA being detected in those cases by spectrophotometric analysis. A possible explanation for this is polymerase chain reaction inhibition, for which there are three likely mechanisms:

direct interaction between inhibitors and polymerase;
interaction of the inhibitor with the DNA; or
interaction with the polymerase during primer extension [21].

It is also possible that the PCR is inhibited by reverse transcriptase [22]. Subsequently, we rejected eight cases as being outliers and extremes.

The analysed population consisted of 44 women and 35 men. Most cases had a negative family history. No statistically significant correlation was observed between exon V expression level and gender or family history (p = 0.2955, p = 0.9003, respectively).

The majority of the investigated tumours were located in the colon. There was no significant correlation between exon V expression level and tumour location (p = 0.9672).

Previously, all examined cases had been histologically classified as tubular or mucinous type. Sixty-nine cases represent tubular type. There was no significant correlation between exon V expression level and histological type of tumour (p = 0.5905).

The exon V expression level was not significantly related to the grade of histological malignancy of the cancer (p = 0.2281).

FJ 194940.1 exon V expression level was compared with several clinicopathological parameters such as depth of tumour invasion (T), presence of lymph node (N) and distant metastases (M), or pTNM stage. There was no significant correlation between the expression level and the comparison parameters (p = 0.9823, 0.7095, 0.2848, 0.7611, respectively).

No statistically significant correlation has been found between the exon V expression level and the presence of lymphocytes in tumour tissue (p = 0.4245). Furthermore, there was no statistically significant correlation between the presence of vessel invasion and the exon V expression level despite a visible tendency towards a lower expression level in a subgroup of cases with vessel invasion presence (p = 0.0697).

All of the findings described above are summarised in Table 1.

Exon V expression level and survival time

To carry out a survival analysis, the entire group was divided into two subgroups based on a median value of the exon V expression level in the entire investigated group. The subgroup described as “low” comprised cases having an expression level lower than the median. The subgroup described as “high” comprised cases showing an expression level equal to or higher than the median. There was a statistically significant difference in survival time probability when comparing the two subgroups (p = 0.0315). Patients with a high exon V expression level show a longer survival time than patients with a low exon V expression level (Fig. 1).

Fig. 1 — Overall survival probability in the patient groups with relatively high and relatively low exon V expression levels

The impact of clinicopathological features on survival time was also analysed. Among these, histological grade, invasion of the intestinal wall, node involvement, distant metastasis, pTNM stage and venous invasion were each significantly related to survival time (univariate analysis, Table 2). Absence of lymph node involvement (N0, p = 0.0008), absence of distant metastasis (M0, p = 0.0000), and lower pTNM stage (pTNM I pTNM II, p = 0.0012) were significantly associated with a longer survival time. Moreover, trends were observed toward a longer survival time in the subgroup of cases of lower malignancy (G1 or G2 stage, p = 0.0673) and lower depth of tumour invasion (T1, T2 p = 0.0562). Likewise, absence of vessel invasion was associated with higher overall survival probability (p = 0.0582). All of the observed dependences are presented in Table 2.

Table 2.

Overall survival analysis according to clinicopathological features and exon V expression level (univariate analysis)

Feature		Number of deaths (%)	p value (log-rank test)
Gender	female	22 (50.0)	0.3137
Gender	male	19 (55.9)	0.3137
Family history	negative	37 (54.4)	0.3924
Family history	positive	4 (40.0)	0.3924
Tumour localization	rectum	17 (56.7)	0.9710
Tumour localization	colon	24 (51.1)	0.9710
Histological type	tubular	36 (52.9)	0.9789
Histological type	mucinous	5 (50.0)	0.9789
Histological grade	G1 or G2	26 (46.4)	0.0673
Histological grade	G3	14 (66.7)	0.0673
Invasion of the intestinal wall	T1 or T2	8 (38.1)	0.0562
Invasion of the intestinal wall	T3 or T4	33 (57.9)	0.0562
Node involvement	N0	15 (36.6)	0.0008
Node involvement	N1 or N2	23 (69.7)	0.0008
Distant metastasis	M0	24 (40.0)	0.0000
Distant metastasis	M1	17 (94.4)	0.0000
pTNM stage	I or II	15 (37.5)	0.0012
pTNM stage	III or IV	26 (68.4)	0.0012
Lymphocytic infiltration	absent	25 (58.1)	0.2299
Lymphocytic infiltration	present	15 (44.1)	0.2299
Vessel invasion	absent	11 (39.3)	0.0582
Vessel invasion	present	30 (60.0)	0.0582
Exon V expression level	high	14 (37.8)	0.0315
Exon V expression level	low	26 (66.7)	0.0315

Open in a new tab

Variables with a p value of less than 0.1 in univariate analysis were chosen to create a Cox regression model. As histological grade, invasion of the intestinal wall, node involvement, distant metastasis, and vessel invasion showed significant correlation with pTNM stage (Table 3), only pTNM stage and exon V expression level were employed to generate the model.

Table 3.

Correlation between TNM stage and other clinicopathological features and exon V expression level

Features	Correlation coefficient	p value
Histological grade (G1 or G2 vs. G3)	0.241	0.041
Invasion of the intestinal wall	0.488	0.000
Node involvement	0.972	0.000
Distant metastasis	0.534	0.000
Vessel invasion	0.367	0.002
Exon V expression level	0.028	0.816

Open in a new tab

Discussion

The main aim of the presented research was to assess any prognostic value of the FJ 194940.1 exon V expression level in colon cancer. To achieve the goal, the expression level assessed by real-time PCR was compared with established prognostic factors and survival time of patients with colorectal cancer.

The analysis conducted shows that exon V expression level is not related significantly with any clinicopathological features in this series of CRC. However, there was a visible tendency to a higher expression level of this exon in cases where tumours do not infiltrate vessels. Furthermore, high exon V expression level was associated with longer survival times. The statistical results obtained indicate that high expression levels of exon V correspond to a risk of death more than two times lower in comparison to cases with a low exon V expression level and, moreover, that the expression level influences the overall survival time independently of any established prognostic factors.

Qualitative expression analysis of the exon V FJ 194940.1 gene transcript has not shown any correlation with clinicopathological features, or any association with survival time [13]. Using real-time PCR, exon V relative expression level in the examined population was shown to be highly diverse, ranging from 0.02 to 18000.36. In normal human tissue, FJ 194940.1 gene is expressed in the kidney [14]. Unpublished data also indicate that in physiological conditions the FJ 194940.1 gene undergoes alternative splicing. Exon V is an invariable element of all detected variants of FJ 194940.1 in colon cancer. In accordance with the above, it is possible that during cancerogenesis the balance between splice variants of this gene is shifted and some isoforms of this gene are more specific for colon cancer. Consequently, quantitative investigation into the expression of separate elements of the FJ 194940.1 transcript could be more useful for colon cancer prognosis.

There is a link between expression of all elements of the part B FJ 194940.1 transcript and low-grade colon cancer [13]. The study presented here shows links between high exon V level expression and lack of vessel infiltration and longer survival time. Exon V is an element of the part B FJ 194940.1 transcript. Consequently, the data may suggest that some part of the FJ 194940.1 gene could play a protective role against the spread of cancer cells and metastasis formation. The exact mechanism through which the gene could exert its effect on CRC progression remains unknown. Some elements of FJ 194940.1 gene expression are associated with better prognosis for patients with colorectal cancer in the analysed series.

The conclusions drawn above stand in contradiction to earlier findings obtained in colon cancer cases [16, 18]. Balcerczak M. et al. [18] suggested that expression of a fragment of the FJ 194940.1 gene transcript in colon cancer is engaged in the process of metastasis formation and could be correlated with worse prognosis for the patient. Expression of fragments of the FJ 194940.1 gene transcript was associated with more advanced tumours, with lymph node metastases and with distant metastases. Quantitative analysis has confirmed these observations. It has shown that the expression level of the FJ 194940.1 gene transcript fragment was higher in cancer with metastases to lymph nodes and distant metastases. Higher levels were observed in more advanced cases, classified as III and IV according to the pTNM classification [16].

The discrepancies described might be explained by the difference in the examined fragment of the FJ 194940.1 transcript. The Bartczak et al. [13] studies took separate exons of the FJ 194940.1 gene into consideration, whereas Balcerczak M. et al. [18] and Balcerczak E. et al. [16] analysed the fragment of its transcript that consists of exon V and part of exon IV. Also, alternative pre-mRNA splicing gives the opportunity to generate multiple transcripts from a single m-RNA precursor, so it is possible to develop two isoform encoding proteins with antagonistic functions. An interesting example of cancer-related regulation by alternative splicing is the BCL-X gene. This gene has two splice variants: long antiapoptotic and short proapoptotic [23]. This is caused by the dephosphorylation of SR proteins, a family of protein factors that regulate alternative splicing (known as trans-acting regulatory factors). Modifications of those proteins by dephosphorylation induce changes in the production of particular isoforms – in this situation, increasing the level of proapoptotic splice variant with a simultaneous loss in the antiapoptotic form [23, 24].

FJ 194940.1 gene expression correlates with cancer progression independently of the analysed clinicopathological parameters.

This study is supported by grant 502-03/3-015-02/502-34-014 – 503/3-015-02/503-06-300 from the Medical University of Łódź, Poland.

References

1.Arnold CN, Goel A, Blum HE, Boland CR. Molecular pathogenesis of colorectal cancer: implications for molecular diagnosis. Cancer. 2005;104:2035–47. doi: 10.1002/cncr.21462. [DOI] [PubMed] [Google Scholar]
2.Goel A, Arnold CN, Niedzwiecki D, et al. Characterization of sporadic colon cancer by patterns of genomic instability. Cancer Res. 2003;63:1608–14. [PubMed] [Google Scholar]
3.Gardina PJ, Clark TA, Shimada B, et al. Alternative splicing and differential gene expression in colon cancer detected by a whole genome exon array. BMC Genomics. 2006;7:325. doi: 10.1186/1471-2164-7-325. [DOI] [PMC free article] [PubMed] [Google Scholar]
4.Venables JP. Aberrant and alternative splicing in cancer. Cancer Res. 2004;64:7647–54. doi: 10.1158/0008-5472.CAN-04-1910. [DOI] [PubMed] [Google Scholar]
5.Brinkman BM. Splice variants as cancer biomarkers. Clin Biochem. 2004;37:584–94. doi: 10.1016/j.clinbiochem.2004.05.015. [DOI] [PubMed] [Google Scholar]
6.Finn L, Dougherty G, Finley G, Meisler A, Becich M, Cooper DL. Alternative splicing of CD44 pre-mRNA in human colorectal tumors. Biochem Biophys Res Commun. 1994;200:1015–22. doi: 10.1006/bbrc.1994.1551. [DOI] [PubMed] [Google Scholar]
7.Goodison S, Urquidi V, Tarin D. CD44 cell adhesion molecules. Mol Pathol. 1999;52:189–96. doi: 10.1136/mp.52.4.189. [DOI] [PMC free article] [PubMed] [Google Scholar]
8.Sternberg LR, Byrd JC, Hansson GC, Liu KF, Bresalier RS. Alternative splicing of the human MUC2 gene. Arch Biochem Biophys. 2004;421:21–33. doi: 10.1016/j.abb.2003.10.002. [DOI] [PubMed] [Google Scholar]
9.Patten LC, Belaguli NS, Baek MJ, Fagan SP, Awad SS, Berger DH. Serum response factor is alternatively spliced in human colon cancer. J Surg Res. 2004;121:92–100. doi: 10.1016/j.jss.2004.02.031. [DOI] [PubMed] [Google Scholar]
10.Huerta S, Srivatsan ES, Venkatesan N, Peters J, Moatamed F, Renner S, Livingston EH. Alternative mRNA splicing in colon cancer causes loss of expression of neural cell adhesion molecule. Surgery. 2001;130:834–3. doi: 10.1067/msy.2001.116415. [DOI] [PubMed] [Google Scholar]
11.Genuardi M, Viel A, Bonora D, et al. Characterization of MLH1 and MSH2 alternative splicing and its relevance to molecular testing of colorectal cancer susceptibility. Hum Genet. 1998;102:15–20. doi: 10.1007/s004390050648. [DOI] [PubMed] [Google Scholar]
12.Pospisil H, Herrmann A, Butherus K, Pirson S, Reich JG, Kemmner W. Verification of predicted alternatively spliced Wnt genes reveals two new splice variants (CTNNB1 and LRP5) and altered Axin-1 expression during tumour progression. BMC Genomics. 2006;7:148. doi: 10.1186/1471-2164-7-148. [DOI] [PMC free article] [PubMed] [Google Scholar]
13.Bartczak-Tomczyk M, Sałagacka A, Mirowski M, Balcerczak E. Investigation of FJ 194940.1 gene alternative splicing in colon cancer and its association with clinicopathological parameters. Exp Ther Med. 2012;3:237–42. doi: 10.3892/etm.2011.378. [DOI] [PMC free article] [PubMed] [Google Scholar]
14.Balcerczak E, Malewski T, Bartczak M, Mirowski M. Alternation of FJ 194940.1 transcript expression after provirus integration in human neoplasm. Int J Integrat Biol. 2011;11:58–63. [Google Scholar]
15.Balcerczak E, Bartkowiak J, Błoński JZ, Robak T, Mirowski M. Expression of gene encoding P65 oncofetal protein in acute and chronic leukemias. Neoplasma. 2002;49:295–9. [PubMed] [Google Scholar]
16.Balcerczak E, Balcerczak M, Mirowski M. Quantitative analysis of the P65 gene expression in patients with coloroctal cancer. Int J Biomed Sci. 2007;3:287–291. [PMC free article] [PubMed] [Google Scholar]
17.Czyz W, Balcerczak E, Rudowicz M, Niewiadomska H, Pasieka Z, Kuzdak K, Mirowski M. Expression of C-ERBB2 and P65 genes and their protein products in follicular neoplasms of thyroid gland. Folia Histochem Cytobiol. 2003;41:91–5. [PubMed] [Google Scholar]
18.Balcerczak M, Balcerczak E, Pasz-Walczak G, Kordek R, Mirowski M. Expression of the p65 gene in patients with colorectal cancer: comparison with some histological typing, grading and clinical staging. Eur J Surg Oncol. 2004;30:266–70. doi: 10.1016/j.ejso.2003.11.006. [DOI] [PubMed] [Google Scholar]
19.Chomczynski P, Sacchi N. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal Biochem. 1987;162:156–9. doi: 10.1006/abio.1987.9999. [DOI] [PubMed] [Google Scholar]
20.Livak KJ, Schmittgen TD. Analysis of relative gene expression data using real-time quantitative PCR and the 2(-Delta Delta C(T)) Method. Methods. 2001;25:402–8. doi: 10.1006/meth.2001.1262. [DOI] [PubMed] [Google Scholar]
21.Opel KL, Chung D, McCord BR. A study of PCR inhibition mechanisms using real time PCR. J Forensic Sci. 2010;55:25–33. doi: 10.1111/j.1556-4029.2009.01245.x. [DOI] [PubMed] [Google Scholar]
22.Chandler DP, Wagnon CA, Bolton H., Jr Reverse transcriptase (RT) inhibition of PCR at low concentrations of template and its implications for quantitative RT-PCR. Appl Environ Microbiol. 1998;64:669–77. doi: 10.1128/aem.64.2.669-677.1998. [DOI] [PMC free article] [PubMed] [Google Scholar]
23.Pajares MJ, Ezponda T, Catena R, Calvo A, Pio R, Montuenga LM. Alternative splicing: an emerging topic in molecular and clinical oncology. Lancet Oncol. 2007;8:349–57. doi: 10.1016/S1470-2045(07)70104-3. [DOI] [PubMed] [Google Scholar]
24.Chalfant CE, Rathman K, Pinkerman RL, Wood RE, Obeid LM, Ogretmen B, Hannun YA. De novo ceramide regulates the alternative splicing of caspase 9 and Bcl-x in A549 lung adenocarcinoma cells. Dependence on protein phosphatase-1. J Biol Chem. 2002;277:12587–95. doi: 10.1074/jbc.M112010200. [DOI] [PubMed] [Google Scholar]

[CIT0001] 1.Arnold CN, Goel A, Blum HE, Boland CR. Molecular pathogenesis of colorectal cancer: implications for molecular diagnosis. Cancer. 2005;104:2035–47. doi: 10.1002/cncr.21462. [DOI] [PubMed] [Google Scholar]

[CIT0002] 2.Goel A, Arnold CN, Niedzwiecki D, et al. Characterization of sporadic colon cancer by patterns of genomic instability. Cancer Res. 2003;63:1608–14. [PubMed] [Google Scholar]

[CIT0003] 3.Gardina PJ, Clark TA, Shimada B, et al. Alternative splicing and differential gene expression in colon cancer detected by a whole genome exon array. BMC Genomics. 2006;7:325. doi: 10.1186/1471-2164-7-325. [DOI] [PMC free article] [PubMed] [Google Scholar]

[CIT0004] 4.Venables JP. Aberrant and alternative splicing in cancer. Cancer Res. 2004;64:7647–54. doi: 10.1158/0008-5472.CAN-04-1910. [DOI] [PubMed] [Google Scholar]

[CIT0005] 5.Brinkman BM. Splice variants as cancer biomarkers. Clin Biochem. 2004;37:584–94. doi: 10.1016/j.clinbiochem.2004.05.015. [DOI] [PubMed] [Google Scholar]

[CIT0006] 6.Finn L, Dougherty G, Finley G, Meisler A, Becich M, Cooper DL. Alternative splicing of CD44 pre-mRNA in human colorectal tumors. Biochem Biophys Res Commun. 1994;200:1015–22. doi: 10.1006/bbrc.1994.1551. [DOI] [PubMed] [Google Scholar]

[CIT0007] 7.Goodison S, Urquidi V, Tarin D. CD44 cell adhesion molecules. Mol Pathol. 1999;52:189–96. doi: 10.1136/mp.52.4.189. [DOI] [PMC free article] [PubMed] [Google Scholar]

[CIT0008] 8.Sternberg LR, Byrd JC, Hansson GC, Liu KF, Bresalier RS. Alternative splicing of the human MUC2 gene. Arch Biochem Biophys. 2004;421:21–33. doi: 10.1016/j.abb.2003.10.002. [DOI] [PubMed] [Google Scholar]

[CIT0009] 9.Patten LC, Belaguli NS, Baek MJ, Fagan SP, Awad SS, Berger DH. Serum response factor is alternatively spliced in human colon cancer. J Surg Res. 2004;121:92–100. doi: 10.1016/j.jss.2004.02.031. [DOI] [PubMed] [Google Scholar]

[CIT0010] 10.Huerta S, Srivatsan ES, Venkatesan N, Peters J, Moatamed F, Renner S, Livingston EH. Alternative mRNA splicing in colon cancer causes loss of expression of neural cell adhesion molecule. Surgery. 2001;130:834–3. doi: 10.1067/msy.2001.116415. [DOI] [PubMed] [Google Scholar]

[CIT0011] 11.Genuardi M, Viel A, Bonora D, et al. Characterization of MLH1 and MSH2 alternative splicing and its relevance to molecular testing of colorectal cancer susceptibility. Hum Genet. 1998;102:15–20. doi: 10.1007/s004390050648. [DOI] [PubMed] [Google Scholar]

[CIT0012] 12.Pospisil H, Herrmann A, Butherus K, Pirson S, Reich JG, Kemmner W. Verification of predicted alternatively spliced Wnt genes reveals two new splice variants (CTNNB1 and LRP5) and altered Axin-1 expression during tumour progression. BMC Genomics. 2006;7:148. doi: 10.1186/1471-2164-7-148. [DOI] [PMC free article] [PubMed] [Google Scholar]

[CIT0013] 13.Bartczak-Tomczyk M, Sałagacka A, Mirowski M, Balcerczak E. Investigation of FJ 194940.1 gene alternative splicing in colon cancer and its association with clinicopathological parameters. Exp Ther Med. 2012;3:237–42. doi: 10.3892/etm.2011.378. [DOI] [PMC free article] [PubMed] [Google Scholar]

[CIT0014] 14.Balcerczak E, Malewski T, Bartczak M, Mirowski M. Alternation of FJ 194940.1 transcript expression after provirus integration in human neoplasm. Int J Integrat Biol. 2011;11:58–63. [Google Scholar]

[CIT0015] 15.Balcerczak E, Bartkowiak J, Błoński JZ, Robak T, Mirowski M. Expression of gene encoding P65 oncofetal protein in acute and chronic leukemias. Neoplasma. 2002;49:295–9. [PubMed] [Google Scholar]

[CIT0016] 16.Balcerczak E, Balcerczak M, Mirowski M. Quantitative analysis of the P65 gene expression in patients with coloroctal cancer. Int J Biomed Sci. 2007;3:287–291. [PMC free article] [PubMed] [Google Scholar]

[CIT0017] 17.Czyz W, Balcerczak E, Rudowicz M, Niewiadomska H, Pasieka Z, Kuzdak K, Mirowski M. Expression of C-ERBB2 and P65 genes and their protein products in follicular neoplasms of thyroid gland. Folia Histochem Cytobiol. 2003;41:91–5. [PubMed] [Google Scholar]

[CIT0018] 18.Balcerczak M, Balcerczak E, Pasz-Walczak G, Kordek R, Mirowski M. Expression of the p65 gene in patients with colorectal cancer: comparison with some histological typing, grading and clinical staging. Eur J Surg Oncol. 2004;30:266–70. doi: 10.1016/j.ejso.2003.11.006. [DOI] [PubMed] [Google Scholar]

[CIT0019] 19.Chomczynski P, Sacchi N. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal Biochem. 1987;162:156–9. doi: 10.1006/abio.1987.9999. [DOI] [PubMed] [Google Scholar]

[CIT0020] 20.Livak KJ, Schmittgen TD. Analysis of relative gene expression data using real-time quantitative PCR and the 2(-Delta Delta C(T)) Method. Methods. 2001;25:402–8. doi: 10.1006/meth.2001.1262. [DOI] [PubMed] [Google Scholar]

[CIT0021] 21.Opel KL, Chung D, McCord BR. A study of PCR inhibition mechanisms using real time PCR. J Forensic Sci. 2010;55:25–33. doi: 10.1111/j.1556-4029.2009.01245.x. [DOI] [PubMed] [Google Scholar]

[CIT0022] 22.Chandler DP, Wagnon CA, Bolton H., Jr Reverse transcriptase (RT) inhibition of PCR at low concentrations of template and its implications for quantitative RT-PCR. Appl Environ Microbiol. 1998;64:669–77. doi: 10.1128/aem.64.2.669-677.1998. [DOI] [PMC free article] [PubMed] [Google Scholar]

[CIT0023] 23.Pajares MJ, Ezponda T, Catena R, Calvo A, Pio R, Montuenga LM. Alternative splicing: an emerging topic in molecular and clinical oncology. Lancet Oncol. 2007;8:349–57. doi: 10.1016/S1470-2045(07)70104-3. [DOI] [PubMed] [Google Scholar]

[CIT0024] 24.Chalfant CE, Rathman K, Pinkerman RL, Wood RE, Obeid LM, Ogretmen B, Hannun YA. De novo ceramide regulates the alternative splicing of caspase 9 and Bcl-x in A549 lung adenocarcinoma cells. Dependence on protein phosphatase-1. J Biol Chem. 2002;277:12587–95. doi: 10.1074/jbc.M112010200. [DOI] [PubMed] [Google Scholar]

PERMALINK

Quantitative analysis of FJ 194940.1 gene expression in colon cancer and its association with clinicopathological parameters

Malwina Bartczak-Tomczyk

Aleksandra Sałagacka

Marek Mirowski

Agnieszka Jeleń

Ewa Balcerczak

Abstract

Aim of the study

Material and methods

Results

Conclusions

Introduction

Material and methods

Materials

Table 1.

RNA isolation

cDNA synthesis

Real-time PCR

Statistical analysis

Results

Exon V expression level and survival time

Fig. 1.

Table 2.

Table 3.

Discussion

References

ACTIONS

PERMALINK

RESOURCES

Cite

Add to Collections

PERMALINK

Quantitative analysis of FJ 194940.1 gene expression in colon cancer and its association with clinicopathological parameters

Malwina Bartczak-Tomczyk

Aleksandra Sałagacka

Marek Mirowski

Agnieszka Jeleń

Ewa Balcerczak

Abstract

Aim of the study

Material and methods

Results

Conclusions

Introduction

Material and methods

Materials

Table 1.

RNA isolation

cDNA synthesis

Real-time PCR

Statistical analysis

Results

Exon V expression level and survival time

Fig. 1.

Table 2.

Table 3.

Discussion

References

ACTIONS

PERMALINK

RESOURCES

Similar articles

Cited by other articles

Links to NCBI Databases