1. Introduction

Globally, pancreatic cancer was the 12th most newly diagnosed cancer in 2020, with 495,773 new cases, and the 7th leading cause of cancer death in 2020 with 466,003 deaths [1,2]. Currently, the only cure for pancreatic cancer is surgery [3], however, only 15–20% of patients have resectable tumours at diagnosis [3]. Furthermore, up to 80% of patients have tumour recurrence following resection [4]. There are few clinically available biomarkers that can effectively guide prognosis and treatment in pancreatic ductal adenocarcinoma (PDAC). Measuring serum levels of cancer antigen 19-9 (CA19-9) can be useful to confirm diagnosis as well as monitor disease recurrence. However, it has a relatively low predictive value and is of limited use in selecting patients for resection [5].

Endoscopic ultrasound guided fine needle aspiration (EUS-FNA) remains the gold standard for the diagnosis of localised PDAC, with a sensitivity of around 85% and specificity of near 100% [6]. Furthermore, it can be used to provide tissue for cytological and even histological diagnosis and can also be utilised for further applications such as KRAS detection [7]. However, it is not currently used to provide prognostic information to guide selection of patients for surgical resection.

In recent years, the molecular landscape of pancreatic cancer has become well defined. The four most commonly mutated genes in pancreatic cancer are KRAS, CDKN2A, TP53, and SMAD4. Mutations in these genes have been associated with oncogenic cellular processes and with prognosis in pancreatic cancer [8]. The KRAS gene encodes a guanosine triphosphatase (GTPase) protein that controls cellular processes by linking membrane growth factor receptors to intracellular signalling pathways and transcription factors. The KRAS gene is mutated in over 90% of PDAC cases [9].

The KRAS mutation is usually a point mutation which frequently occurs on codon 12 of exon 2, affecting the first or second nucleotide, but can also affect other codons and exons such as codon 13 and 61. The normal or wild-type sequence is GGT encoding glycine, and it is present in 8–12% of PDAC [10]. The most common mutation subtype is G12D, present in 40% of patients, whereby a GAT sequence is coded, producing aspartic acid [10]. G12V subtype refers to a GTT replacement sequence producing valine, and G12R refers to a CGT replacement sequence producing arginine, and these are present in 33% and 15% of PDAC cases, respectively [10].

Detection of KRAS does not currently have a role in screening or diagnosis of pancreatic cancer due to difficulty standardizing sampling, transportation, extraction and detection. However, many studies have demonstrated cytopathology with KRAS on EUS-FNA materials has a higher sensitivity, specificity and accuracy of PDAC diagnosis compared to cytopathology alone [10]. Furthermore, liquid biopsies which detect circulating tumour cells and cell-free circulating tumour DNA (ctDNA) have been heavily investigated diagnostically and prognostically, with varying results [10,11].

Many studies have investigated the association between KRAS mutation and PDAC patient survival, predominantly in patients with early-stage, resectable disease. Most studies found that KRAS mutation was significantly associated with shorter overall survival, although a small number of studies found no statistically significant correlation [12,13,14,15]. The association between KRAS mutation and survival in PDAC patients with advanced unresectable disease has also been assessed. EUS-FNA was the main source of tissue for KRAS detection in this patient cohort [16,17,18]. Ogura et al. analysed 242 patients with unresectable pancreatic cancer and found that those in the KRAS mutation group had a significantly shorter survival compared to the wild-type group [16]. Conversely, a recent study by on 219 patients with advanced PDAC found that there was no significant difference in survival between the mutant KRAS and KRAS wild-type groups [18]. However, overall, as demonstrated in a recent meta-analysis, patients with KRAS mutation had poorer overall survival [19].

When considering the different mutant KRAS subtypes, G12D is both the most frequently occurring KRAS mutation subtype (36.9–67%) and also the subtype that is most commonly reported as being associated with poorer survival [12,13,14,15,16,18,20,21]. For example, Qian et al. found that KRAS G12D subtype patients had an overall median survival of 15.3 months compared to 24.8 months in patients without the KRAS G12D subtype [15] (n = 356). However, the KRAS G12A and G12R subtypes have also been reported as being associated with a reduction in patient survival [12,16], while other investigators have been unable to demonstrate any correlation between a particular KRAS subtype and survival [17].

Given the heterogeneity of these results, we sought to assess the correlation between the KRAS G12D mutation subtype and survival in pancreatic cancer patients across all clinical stages using tissue biopsies obtained predominantly via EUS-FNA.

2. Methods

2.1. Ethics Statement

This retrospective cohort study was approved by the Monash Health Human Research Ethics Committee (Monash Health HREC Ref: 17387L). The cohort was comprised of patients who had previously had KRAS mutations analysis performed on EUS-FNA or resection specimens. The patients had either provided tissue as part of the Victorian Pancreatic Cancer Biobank and various sub studies associated with this (Monash Health HREC Ref: 15450A) or were being screened for enrolment in a prospective cohort study examining the use of panitumumab as second or subsequent line therapy in advanced KRAS wild-type pancreatic cancer (Monash Health HREC Ref: 16584A) [22]. All patient information was stored in a confidential and de-identified manner.

2.2. Data and Sample Collection

We included all consenting patients from 2012 to 2020 with KRAS mutation data. Demographic data, date and method of diagnosis, treatment details and survival were reviewed. Clinical stage was established via review of multi-disciplinary team meeting documentation. In general, clinical staging was determined on anatomical criteria using the NCCN Pancreatic Adenocarcinoma guidelines (2016) [23,24]. These guidelines specify criteria such as degree of tumour contact or invasion on the superior mesenteric artery, coeliac artery, or common hepatic artery, to distinguish between resectable, borderline resectable, locally advanced or metastatic pancreatic disease.

KRAS mutation analysis was performed either on EUS FNA specimens or from tissue taken from pancreatic resections (either a snap frozen core biopsy of the tumour taken immediately after resection or from archival formalin fixed paraffin blocks later retrieved from the pathology department). For patients undergoing EUS-FNA an additional biopsy was snap frozen and stored at −80°C or in liquid nitrogen in the Victorian Pancreatic Cancer Biobank (Monash Health HREC Ref: 15450A) or the Monash Surgical Oncology Biobank (Monash Health HREC Ref: 13058A).

DNA was extracted from patient biopsy samples via homogenization in a Buffer RLT plus AllPrep DNA/RNA Universal Kit (Qiagen, Hilden, Germany) as per the manufacturer’s protocol. The isolation of gDNA from FFPE tissue was performed on 5 × 10 micron-thick sections using the ReliaPrep FFPE gDNA Miniprep System (Promega, Madison, WI, USA). The quality and quantity of gDNA were determined on a NanoDrop Spectrophotometer (Thermo Fisher Scientific, Waltham, MA, USA) and Qubit Fluorometer (ThermoScientific), and TapeStation (Agilent, St. Clara, CA, USA). gDNA (25–50 ng) was subjected to the KRAS XL StripAssay^® (ViennaLab Diagnostics GmbH, Wien, Austria). Mutations were objectively scored using StripAssay Evaluator software. For a small number of patients, KRAS mutation was determined using the TruSight Oncology 500 (TSO-500) gene panel (Illumina, San Diego, CA, USA).

2.3. Statistical Analysis

Survival was measured from date of first tissue diagnosis (either EUS-FNA or surgical resection, whichever came first) until death or censoring date defined as the last known follow-up. Treatment groups were based on if patients received resection with curative intent, chemotherapy and/or radiotherapy without surgery or supportive care only. In patients who received surgery, we further recorded lymph node status, tumour location, resection margin clearance and whether or not adjuvant or neoadjuvant therapy was administered.

A chi-squared test, chi-squared test with Yates’ continuity correction, and Fisher’s exact test were used to assess independent categorical variables. A Mann—Whitney U test was used to compare differences in age. Kaplan-Meier curves were generated for median survival within individual groups, and these were compared using the log-rank test for univariate analysis. KRAS mutant was compared with KRAS wild-type, and the G12D subtype was compared with non-G12D patients, which consists of all other mutant KRAS subtypes and KRAS wild-types combined. Multivariate analysis only included KRAS mutation as a whole, and also the G12D, G12V and G12R subtypes individually, and used covariates associated with survival on univariate analysis (defined by p < 0.1) and was conducted using the Cox proportional hazards regression model. The sample method (FNA vs. resection) was excluded from multivariate analysis as this was not considered clinically relevant to patient survival.

Statistical significance was defined at p < 0.05. All statistical analyses were performed using GraphPad Prism Version 9.1.1 (GraphPad Software, San Diego, CA, USA) and IBM SPSS Statistics 27 (IBM, Armonk, NY, USA).

3. Results

3.1. Patient Characteristics at Baseline

Baseline characteristics are shown in Table 1. A total of 231 patients had KRAS mutation status available for analysis (109 males, 122 females, IQR = 14.02). Of these, 202 patients had a KRAS mutation (87.4%) and 29 patients were KRAS wild-type (12.6%). Furthermore, 194 patients had a KRAS mutation detected through EUS-FNA (84.0%) with a KRAS mutation rate of 87.1% (169/194), whilst 37 patients had a KRAS mutation detected through assessment of resection specimens (16.0%) with a mutation rate of 89.2% (33/37). There was no difference in the KRAS detection rate depending on the method of tissue acquisition, either EUS-FNA or surgical resection (p = 0.9374).

The 3 most frequently occurring KRAS mutation subtypes were G12D (93 patients, 40.3%), G12V (64 patients, 27.7%) and G12R (24 patients, 10.4%). (Table 2) There were 138 patients in total who were not KRAS G12D, including KRAS wild-type patients (59.5%).

There was no significant correlation between KRAS mutation and clinical stage at diagnosis (p = 0.1627; df = 3). Further, the G12D mutation subtype was also not significantly associated with clinical stage at diagnosis (p = 0.500, df = 3) (Table 1).

For patients who underwent resection, lymph node status (positive or negative), tumour location within pancreas (head or distal), neoadjuvant therapy (yes or no), resection margin (clear or positive) and adjuvant therapy (yes or no) information was present for 50, 53, 51, 53 and 51 patients, respectively, due to loss of follow-up (see Table 3). In patients who received surgery, there was no correlation between KRAS mutation status or G12D subtype and surgical parameters such as lymph node status (p = 0.8719, 95% CI 0.6179–2.760) and tumour location (p = 0.9274, RR 1.170 95% CI 0.6013–2.694) (Table 3).

3.2. Survival Analysis for the Entire Cohort

Multivariate analysis showed that only NCCN clinical stage and treatment modality were significantly associated with overall survival (Table 4). Across the whole population, patients with a KRAS mutation did not have significantly worse survival compared to KRAS wild-type patients (296 vs. 420 days, p = 0.843; HR 1.050 95% CI (0.646–1.709)). The G12D mutation subtype was also not associated with poorer survival compared to non-G12D PDAC patients (which included both other forms of mutant KRAS and KRAS wild-type) (p = 0.107; HR 1.293 95% CI (0.946–1.767)). Similarly, neither G12V nor G12R were associated with changes in patient survival.

In patients who received surgery, lymph node positivity and tumour location were associated with survival on univariate analysis but not on multivariate analysis. Neoadjuvant therapy, resection margins and adjuvant therapy were not associated with survival in this cohort (Table 5).

3.3. Survival Analysis by NCCN Stage and Treatment Modality and KRAS Mutation Status

There was no significant difference in overall survival between KRAS mutant and wild-type patients in any clinical stage of disease, however, in the resectable group, G12D patients had a significantly shorter median survival time of 356 days compared to non-G12D PDAC patients (which included both other forms of mutant KRAS and KRAS wild-type) (median survival 810 days) on both univariate analysis (p = 0.0168; HR 2.053 95% CI (1.139–3.702)) and multivariate analysis (p = 0.019; HR 1.991 95% CI (1.121–3.537)) (Table 6 and Figure 1). There were no associations between survival and G12D subtype in any of the other stages of disease, namely, borderline resectable, locally advanced and metastatic.

Similarly, with respect to the treatment modality, there was also no statistically significant difference in overall survival between KRAS mutant and wild-type patients in patients in any of the treatment groups: surgery, chemotherapy/radiotherapy and best supportive care. However, G12D patients who underwent surgery had significantly shorter median survival of 462 days compared to all non-G12D patients (median survival 1084 days) on univariate analysis (0.0221; HR 2.000 95% CI (1.079–3.707)) although not on multivariate analysis (0.254; HR 1.471 95% CI (0.758–2.855)) (See Figure 1). Within the chemotherapy/radiotherapy group and also within the supportive care group, there was no association between KRAS G12D subtype and survival.

These data suggest that the KRAS G12D mutation subtype is associated with poorer survival within NCCN resectable patients. Due to the low numbers of G12V and G12R patients within each clinical stage and treatment modality cohort, no attempt was made to assess for correlations between survival and the presence of these subtypes.

4. Discussion

In this retrospective cohort study examining the correlation between the presence of a KRAS G12D mutation subtype and prognosis in PDAC across all stages of disease, we found that the presence of a KRAS G12D mutation was associated with reduced survival in those with resectable disease. There was also a suggestion (on univariate analysis only) of reduced survival in patients with a KRAS G12D mutation who underwent resection, however, after adjusting for potential confounders, this was no longer statistically significant (on multivariate analysis). A larger sample size may help clarify this further. There was no association between KRAS G12D mutation and the clinical stage of disease at presentation. Further, we could not demonstrate a statistically significant association between the presence of a KRAS G12D mutation subtype and survival in other clinical stages of disease or with other treatment modalities.

Our study is unique in a number of ways. Firstly, although we predominantly used EUS to assess KRAS mutation status, we also included analysis of resection specimens (in patients who had not undergone EUS-FNA) allowing us to assess the association between KRAS mutation and subtype across all stages of disease and in all treatment groups. Furthermore, we found that 87.4% of patients had a KRAS mutation, which reflects the approximately 90% frequency reported in current literature [9]. In addition, G12D is typically cited as occurring in 40% of PDAC patients, G12V usually occurs in 33% of patients, and G12R typically occurs in 15% of patients [10]. Our cohort had 40.3% G12D, 27.7% G12V and 10.4% G12R. As such, our cohort is a representative sample of a PDAC population from a KRAS mutation frequency perspective. Previous studies which have used EUS-FNA to assess KRAS mutation status have often reported significantly lower rates of KRAS mutation detection suggesting significant sampling error [12,13,14]. The fact that we utilized an additional snap frozen biopsy for molecular analysis probably accounts for this difference. If EUS-FNA is to be used to guide treatment decisions based on molecular analyses, it is important that the information provided is indeed reliable and reflective of the tumour.

Secondly, our study represents the first time that the prevalence of KRAS mutations has been simultaneously analysed across all clinical stages of disease allowing us to assess any potential associations between KRAS mutations and both stage at presentation and survival. Most previous studies assessed either only resected patients [25] or advanced unresectable disease [19]. Furthermore, although some previous studies which focused on resected patients considered TNM as an independent predictor of survival [19,25], we chose to use the NCCN staging system [26,27]. The rationale for this is that the TNM staging system requires accurate assessment of lymph nodes status and this is only available for the 20% of patients who undergo resection, whereas the NCCN staging system can be applied to the whole population. We hypothesized that given that treatment options such as surgery or chemotherapy remain the most important prognosticators in PDAC, any association between KRAS mutation and survival may be mediated by differences in the prevalence of KRAS mutations and/or subtypes in the various NCCN clinical stages at diagnosis. However, as demonstrated above, there was in fact no association between KRAS mutation and/or subtype and clinical stage at presentation. Moreover, there was no association between G12D mutation and the presence of lymph node metastases within the resected cohort, further suggesting that the deleterious effect of G12D is not mediated through its impact on stage at diagnosis, even in those with resectable disease.

The G12D subtype has previously been shown to be associated with poorer prognosis, however, the literature is somewhat conflicting [12,13,14,15,17,19,20]. The strongest evidence for G12D being a marker of poor prognosis comes from studies of patients with operable disease, whereas the evidence for advanced disease is less clear cut. Our data support this. Since G12D is present in 40% of PDAC patients [10], this finding has potentially important clinical implications. For patients who are considered anatomically resectable, but who are marginal surgical candidates due to age and comorbidities, KRAS mutation assessment could be useful to guide treatment decisions. The fact that KRAS mutation subtype can be reliably assessed via EUS-FNA enables this information to be available prior to considering surgery.

The reason for exploring KRAS mutation status as a prognostic biomarker rather than any other potentially useful biomarkers, such as Ki67, is that these patients were being screened for potential inclusion in a clinical study of EGFR inhibition in KRAS wild-type pancreatic cancer [22]. The recent introduction of targeted therapies directed at specific KRAS subtypes highlights the fact that it will become increasingly important to be able assess prognostic and predictive biomarkers using EUS-FNA biospecimens. For example, targeting G12C has recently demonstrated significant anti-tumour activity in clinical trials, some of which included PDAC patients [28]. Sotorasib, a G12C inhibitor, has been approved for clinical use in non-small-cell lung cancer, after promising phase I and II trials [28,29]. Another approach includes siG12D-LODER™, an siRNA which targets KRAS loaded into a biodegradable polymetric matrix [30]. Early phase clinical trials in PDAC have reported it is well tolerated, with promising signs of efficacy [31]. Engineered inhibitory exosomes have proven to be effective in PDAC preclinical models [32]. All these approaches rely on accurate assessment of the subtype status prior to surgery. We have convincingly demonstrated that EUS-FNA can be used to assess KRAS subtype status in patients with PDAC.

There are a number of limitations in our study. These include that it is from a single center and has a relatively small sample size for survival analysis. The latter may have contributed to the failure to demonstrate an association between the presence of a KRAS mutation and decreased survival (compared to wild-type disease), despite the positive findings of previous papers. In addition, it was difficult to solely compare G12D subtype survival to KRAS wild-type. The relatively small sample size guided our choice to focus on KRAS G12D as the most prevalent subtype and to compare this subtype to all other subtypes combined, including G12R, G12V and wild-type. A comparison between each of the various subtypes individually was not possible with this sample size and may have led to the problem of multiple testing. However, comparing G12D to non G12D includes all patients rather than just wild-type patients and is used in existing studies [11,19]. Further, we know that adjuvant therapy, lymph node status and surgical margins are associated with survival outcomes [33,34,35], and the fact that none of these factors were associated with survival on multivariate analysis further demonstrates the lack of power in our study. Finally, the exact details of the chemotherapy received were not reported as many patients had been referred from other centers for diagnostic biopsy and returned to the referring center for chemotherapy. Furthermore, the chemotherapy regimens used were too heterogenous and, given the sample size, were unlikely to have provided statistically meaningful results when examined individually. Time to recurrence was also not reported as it is difficult to collect in retrospective studies, especially as many patients returned to their referring centers for ongoing treatment.

A potential perceived limitation of our study was that only 37 out of the 63 resected specimens had KRAS mutation analysis performed on the specimens themselves, with the rest having KRAS analysis conducted on EUS-FNA samples prior to surgery. It could be argued that due to the small volume of material obtained, EUS-FNA evaluation may not be able to reflect tumour heterogeneity as well as resection specimens. However, the presence of more than one KRAS mutation subtype within the same tumour has almost never been reported even in resection specimens, demonstrating that tumour heterogeneity is not a relevant consideration with respect to KRAS mutation subtype. This is probably because an activating KRAS mutation is known to occur early in the dysplasia-carcinoma pathway and is therefore likely to be present in virtually every malignant cell.

Given the conflicting results in the literature, further large cohorts may be required to definitively establish the nature of any subtle correlation between NCCN stage and/or prognosis and KRAS mutation subtype, particularly G12D, in PDAC. A meta-analysis assessing the association between specific KRAS subtypes such as G12D and prognosis in different stages of disease is also warranted given the potential importance of this prognostic information.

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Enlarge this image.

Figure 1. Kaplan Meier curves and respective numbers at risk. G12D subtype associated with poorer survival in patients NCCN staged as resectable. (a) G12D subtype associated with poorer survival in patients NCCN staged as operable. (b) G12D subtype associated with poorer survival in patients who received surgery. G12D absent includes both other KRAS subtypes and KRAS wild-type.

References

1. Ferlay, J.E.M.; Lam, F.; Colombet, M.; Mery, L.; Piñeros, M.; Znaor, A.; Soerjomataram, I.; Bray, F. Global Cancer Observatory: Cancer Today; International Agency for Research on Cancer: Lyon, France, 2020; Available online: https://gco.iarc.fr/today (accessed on 6 June 2020).

2. Sung, H.; Ferlay, J.; Siegel, R.L.; Laversanne, M.; Soerjomataram, I.; Jemal, A.; Bray, F. Global Cancer Statistics 2020: GLOBOCAN Estimates of Incidence and Mortality Worldwide for 36 Cancers in 185 Countries. CA Cancer J. Clin.; 2021; 71, pp. 209-249. [DOI: https://dx.doi.org/10.3322/caac.21660] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/33538338]

3. Vincent, A.; Herman, J.; Schulick, R.; Hruban, R.H.; Goggins, M. Pancreatic cancer. Lancet; 2011; 378, pp. 607-620. [DOI: https://dx.doi.org/10.1016/S0140-6736(10)62307-0]

4. Dunne, R.F.; Hezel, A.F. Genetics and Biology of Pancreatic Ductal Adenocarcinoma. Hematol. Clin. N. Am.; 2015; 29, pp. 595-608. [DOI: https://dx.doi.org/10.1016/j.hoc.2015.04.003] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/26226899]

5. Tempero, M.A.; Malafa, M.P.; Al-Hawary, M.; Asbun, H.; Bain, A.; Behrman, S.W.; Benson, A.B.; Binder, E.; Cardin, D.B.; Cha, C. et al. Pancreatic Adenocarcinoma, Version 2.2017, NCCN Clinical Practice Guidelines in Oncology. J. Natl. Compr. Cancer Netw.; 2017; 15, pp. 1028-1061. [DOI: https://dx.doi.org/10.6004/jnccn.2017.0131]

6. Fuccio, L.; Hassan, C.; Laterza, L.; Correale, L.; Pagano, N.; Bocus, P.; Fabbri, C.; Maimone, A.; Cennamo, V.; Repici, A. et al. The role of K-ras gene mutation analysis in EUS-guided FNA cytology specimens for the differential diagnosis of pancreatic solid masses: A meta-analysis of prospective studies. Gastrointest. Endosc.; 2013; 78, pp. 596-608. [DOI: https://dx.doi.org/10.1016/j.gie.2013.04.162]

7. Kamisawa, T.; Wood, L.D.; Itoi, T.; Takaori, K. Pancreatic cancer. Lancet; 2016; 388, pp. 73-85. [DOI: https://dx.doi.org/10.1016/S0140-6736(16)00141-0]

8. Cicenas, J.; Kvederaviciute, K.; Meskinyte, I.; Meskinyte-Kausiliene, E.; Skeberdyte, A.; Cicenas, J. KRAS, TP53, CDKN2A, SMAD4, BRCA1, and BRCA2 Mutations in Pancreatic Cancer. Cancers; 2017; 9, 42. [DOI: https://dx.doi.org/10.3390/cancers9050042]

9. Singhi, A.D.; George, B.; Greenbowe, J.R.; Chung, J.; Suh, J.; Maitra, A.; Klempner, S.J.; Hendifar, A.; Milind, J.M.; Golan, T. et al. Real-Time Targeted Genome Profile Analysis of Pancreatic Ductal Adenocarcinomas Identifies Genetic Alterations That Might Be Targeted with Existing Drugs or Used as Biomarkers. Gastroenterology; 2019; 156, pp. 2242-2253. e4. [DOI: https://dx.doi.org/10.1053/j.gastro.2019.02.037]

10. Buscail, L.; Bournet, B.; Cordelier, P. Role of oncogenic KRAS in the diagnosis, prognosis and treatment of pancreatic cancer. Nat. Rev. Gastroenterol. Hepatol.; 2020; 17, pp. 153-168. [DOI: https://dx.doi.org/10.1038/s41575-019-0245-4]

11. Buscail, E.; Maulat, C.; Muscari, F.; Chiche, L.; Cordelier, P.; Dabernat, S.; Alix-Panabières, C.; Buscail, L. Liquid Biopsy Approach for Pancreatic Ductal Adenocarcinoma. Cancers; 2019; 11, 852. [DOI: https://dx.doi.org/10.3390/cancers11060852]

12. Kawesha, A.; Ghaneh, P.; Andrén-Sandberg, Å.; Ögraed, D.; Skar, R.; Dawiskiba, S.; Evans, J.D.; Campbell, F.; Lemoine, N.; Neoptolemos, J.P. K-ras oncogene subtype mutations are associated with survival but not expression of p53, p16INK4A, p21WAF-1, cyclin D1, erbB-2 and erbB-3 in resected pancreatic ductal adenocarcinoma. Int. J. Cancer; 2000; 89, pp. 469-474. [DOI: https://dx.doi.org/10.1002/1097-0215(20001120)89:6<469::AID-IJC1>3.0.CO;2-L]

13. Shin, S.H.; Kim, S.C.; Hong, S.-M.; Kim, Y.H.; Song, K.-B.; Park, K.-M.; Lee, Y.-J. Genetic Alterations of K-ras, p53, c-erbB-2, and DPC4 in Pancreatic Ductal Adenocarcinoma and Their Correlation with Patient Survival. Pancreas; 2013; 42, pp. 216-222. [DOI: https://dx.doi.org/10.1097/MPA.0b013e31825b6ab0] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/23344532]

14. Rachakonda, P.S.; Bauer, A.S.; Xie, H.; Campa, D.; Rizzato, C.; Canzian, F.; Beghelli, S.; Greenhalf, W.; Costello, E.; Schanne, M. et al. Somatic Mutations in Exocrine Pancreatic Tumors: Association with Patient Survival. PLoS ONE; 2013; 8, e60870. [DOI: https://dx.doi.org/10.1371/journal.pone.0060870] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/23565280]

15. Qian, Z.R.; Rubinson, D.A.; Nowak, J.A.; Morales-Oyarvide, V.; Dunne, R.F.; Kozak, M.M.; Welch, M.W.; Brais, L.K.; Da Silva, A.; Li, T. et al. Association of Alterations in Main Driver Genes with Outcomes of Patients with Resected Pancreatic Ductal Adenocarcinoma. JAMA Oncol.; 2018; 4, e173420. [DOI: https://dx.doi.org/10.1001/jamaoncol.2017.3420] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/29098284]

16. Ogura, T.; Yamao, K.; Hara, K.; Mizuno, N.; Hijioka, S.; Imaoka, H.; Sawaki, A.; Niwa, Y.; Tajika, M.; Kondo, S. et al. Prognostic value of K-ras mutation status and subtypes in endoscopic ultrasound-guided fine-needle aspiration specimens from patients with unresectable pancreatic cancer. J. Gastroenterol.; 2012; 48, pp. 640-646. [DOI: https://dx.doi.org/10.1007/s00535-012-0664-2]

17. Boeck, S.; Jung, A.; Laubender, R.P.; Neumann, J.; Egg, R.; Goritschan, C.; Ormanns, S.; Haas, M.; Modest, D.P.; Kirchner, T. et al. KRAS mutation status is not predictive for objective response to anti-EGFR treatment with erlotinib in patients with advanced pancreatic cancer. J. Gastroenterol.; 2013; 48, pp. 544-548. [DOI: https://dx.doi.org/10.1007/s00535-013-0767-4]

18. Bournet, B.; Muscari, F.; Buscail, C.; Assenat, E.; Barthet, M.; Hammel, P.; Selves, J.; Guimbaud, R.; Cordelier, P.; Buscail, L. KRAS G12D Mutation Subtype Is A Prognostic Factor for Advanced Pancreatic Adenocarcinoma. Clin. Transl. Gastroenterol.; 2016; 7, e157. [DOI: https://dx.doi.org/10.1038/ctg.2016.18]

19. Gu, Y.; Ji, Y.; Jiang, H.; Qiu, G. Clinical Effect of Driver Mutations of KRAS, CDKN2A/P16, TP53, and SMAD4 in Pancreatic Cancer: A Meta-Analysis. Genet. Test. Mol. Biomarkers; 2020; 24, pp. 777-788. [DOI: https://dx.doi.org/10.1089/gtmb.2020.0078]

20. Hendifar, A.E.; Blais, E.M.; Ng, C.; Thach, D.; Gong, J.; Sohal, D.; Chung, V.; Sahai, V.; Fountzilas, C.; Mikhail, S. et al. Comprehensive analysis of KRAS variants in patients (pts) with pancreatic cancer (PDAC): Clinical/molecular correlations and real-world outcomes across standard therapies. J. Clin. Oncol.; 2020; 38, 4641. [DOI: https://dx.doi.org/10.1200/JCO.2020.38.15_suppl.4641]

21. Philip, P.A.; Azar, I.; Xiu, J.; Hall, M.J.; Hendifar, A.E.; Lou, E.; Hwang, J.J.; Gong, J.; Feldman, R.; Ellis, M. et al. Molecular Characterization of KRAS Wild-type Tumors in Patients with Pancreatic Adenocarcinoma. Clin. Cancer Res.; 2022; 28, pp. 2704-2714. [DOI: https://dx.doi.org/10.1158/1078-0432.CCR-21-3581]

22. Lundy, J.; Harris, M.; Zalcberg, J.; Zimet, A.; Goldstein, D.; Gebski, V.; Borsaru, A.; Desmond, C.; Swan, M.; Jenkins, B.J. et al. EUS-FNA Biopsies to Guide Precision Medicine in Pancreatic Cancer: Results of a Pilot Study to Identify KRAS Wild-Type Tumours for Targeted Therapy. Front. Oncol.; 2021; 11, 770022. [DOI: https://dx.doi.org/10.3389/fonc.2021.770022] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/34956889]

23. Tempero, M.A.; Arnoletti, J.P.; Behrman, S.W.; Ben-Josef, E.; Benson Iii, A.B.; Casper, E.S.; Cohen, S.J.; Czito, B.; Ellenhorn, J.D.I.; Hawkins, W.G. et al. Pancreatic adenocarcinoma, version 2.2012: Featured updates to the NCCN guidelines. JNCCN J. Natl. Compr. Cancer Netw.; 2012; 10, pp. 703-713. [DOI: https://dx.doi.org/10.6004/jnccn.2012.0073] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/22679115]

24. Isaji, S.; Mizuno, S.; Windsor, J.A.; Bassi, C.; Castillo, C.F.-D.; Hackert, T.; Hayasaki, A.; Katz, M.H.; Kim, S.-W.; Kishiwada, M. et al. International consensus on definition and criteria of borderline resectable pancreatic ductal adenocarcinoma 2017. Pancreatology; 2018; 18, pp. 2-11. [DOI: https://dx.doi.org/10.1016/j.pan.2017.11.011] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/29191513]

25. McIntyre, C.A.; Lawrence, S.A.; Richards, A.L.; Chou, J.F.; Wong, W.; Capanu, M.; Berger, M.F.; Donoghue, M.T.A.; Yu, K.H.; Varghese, A.M. et al. Alterations in driver genes are predictive of survival in patients with resected pancreatic ductal adenocarcinoma. Cancer; 2020; 126, pp. 3939-3949. [DOI: https://dx.doi.org/10.1002/cncr.33038]

26. Kulkarni, N.M.; Soloff, E.V.; Tolat, P.P.; Sangster, G.P.; Fleming, J.B.; Brook, O.R.; EHecht, l.M.; Kastrinos, F.; Wang, Z.J.; Soloff, E.V. et al. White paper on pancreatic ductal adenocarcinoma from society of abdominal radiology’s disease-focused panel for pancreatic ductal adenocarcinoma: Part I, AJCC staging system, NCCN guidelines, and borderline resectable disease. Abdom. Radiol.; 2020; 45, pp. 716-728. [DOI: https://dx.doi.org/10.1007/s00261-019-02289-5] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/31748823]

27. National Comprehensive Cancer Network. Pancreatic Adenocarcinoma (Version 1.2022). 2022; Available online: https://www.nccn.org/professionals/physician_gls/pdf/pancreatic.pdf (accessed on 6 September 2022).

28. Hong, D.S.; Fakih, M.G.; Strickler, J.H.; Desai, J.; Durm, G.A.; Shapiro, G.I.; Falchook, G.S.; Price, T.J.; Sacher, A.; Denlinger, C.S. et al. KRAS(G12C) Inhibition with Sotorasib in Advanced Solid Tumors. N. Engl. J. Med.; 2020; 383, pp. 1207-1217. [DOI: https://dx.doi.org/10.1056/NEJMoa1917239]

29. Skoulidis, F.; Li, B.T.; Dy, G.K.; Price, T.J.; Falchook, G.S.; Wolf, J.; Italiano, A.; Schuler, M.; Borghaei, H.; Barlesi, F. et al. Sotorasib for Lung Cancers with KRAS p.G12C Mutation. N. Engl. J. Med.; 2021; 384, pp. 2371-2381. [DOI: https://dx.doi.org/10.1056/NEJMoa2103695]

30. Yuan, T.L.; Fellmann, C.; Lee, C.-S.; Ritchie, C.D.; Thapar, V.; Lee, L.C.; Hsu, D.J.; Grace, D.; Carver, J.O.; Zuber, J. et al. Development of siRNA Payloads to Target KRAS-Mutant Cancer. Cancer Discov.; 2014; 4, pp. 1182-1197. [DOI: https://dx.doi.org/10.1158/2159-8290.CD-13-0900]

31. Golan, T.; Khvalevsky, E.Z.; Hubert, A.; Gabai, R.M.; Hen, N.; Segal, A.; Domb, A.; Harari, G.; Ben David, E.; Raskin, S. et al. RNAi therapy targeting KRAS in combination with chemotherapy for locally advanced pancreatic cancer patients. Oncotarget; 2015; 6, pp. 24560-24570. [DOI: https://dx.doi.org/10.18632/oncotarget.4183]

32. Kamerkar, S.; LeBleu, V.S.; Sugimoto, H.; Yang, S.; Ruivo, C.; Melo, S.; Lee, J.J.; Kalluri, R. Exosomes facilitate therapeutic targeting of oncogenic KRAS in pancreatic cancer. Nature; 2017; 546, pp. 498-503. [DOI: https://dx.doi.org/10.1038/nature22341]

33. Loveday, B.P.T.; Lipton, L.; Thomson, B.N.J. Pancreatic cancer. Aust. J. Gen. Pract.; 2019; 48, pp. 826-831. [DOI: https://dx.doi.org/10.31128/AJGP-06-19-4957] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/31774983]

34. Oba, A.; Ho, F.; Bao, Q.R.; Al-Musawi, M.H.; Schulick, R.D.; Del Chiaro, M. Neoadjuvant Treatment in Pancreatic Cancer. Front. Oncol.; 2020; 10, 245. [DOI: https://dx.doi.org/10.3389/fonc.2020.00245] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/32185128]

35. Tummers, W.S.; Groen, J.V.; Mulder, B.G.S.; Farina-Sarasqueta, A.; Morreau, J.; Putter, H.; Van De Velde, C.J.; Vahrmeijer, A.L.; Bonsing, B.A.; Mieog, J.S. et al. Impact of resection margin status on recurrence and survival in pancreatic cancer surgery. Br. J. Surg.; 2019; 106, pp. 1055-1065. [DOI: https://dx.doi.org/10.1002/bjs.11115] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/30883699]