Oral versus intravenous vinorelbine: clinical safety profile

Gebbia, Vittorio; Puozzo, C.

doi:10.1517/14740338.4.5.915

Cited by 65 publications

(51 citation statements)

References 56 publications

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“…The serum levels of commonly administered spindle poisons, such as vincristine, vindesine, vinblastine, vinorelbine and taxol, are higher only within a short period of time after administration. 20,[31][32][33] Prolonged exposure to rather low serum levels may lead to induction of apoptosis only in those tumors that are highly sensitive to spindle poisons. However, we noted that AML cells are not able to undergo a sustained mitotic block even in the presence of high doses of spindle poison as evidenced in its extreme form by the finding of sister-chromatid separation in the presence of spindle disruption.…”

Section: Discussionmentioning

confidence: 99%

BubR1 is frequently repressed in acute myeloid leukemia and its re-expression sensitizes cells to antimitotic therapy

Schnerch¹,

Schmidts²,

Follo³

et al. 2013

Haematologica

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ABSTRACT© F e r r a t a S t o r t i F o u n d a t i o n 2 0 1 3 blasts investigated. By performing functional studies both in non-responsive myeloblastic and responsive lymphoblastic cells, we investigated how reconstitution of the SAC and interference with SAC activity translate into response to spindle poison. Using live-cell imaging, retrovirus-delivered inducible knockdown and overexpression, we demonstrate that re-expression of BubR1 in myeloblastic cells confers an improved response to spindle poison. Methods Cell culturesCell lines were cultured as described in the DSMZ (Human and Animal Cell Lines Database, Braunschweig, Germany) datasheets. Synchronization procedures, interference with microtubule kinetics, proteasome inhibition and antibiotic selection were performed as outlined in the Online Supplementary Appendix.Primary blasts from AML patients were isolated and cultured as described in the Online Supplementary Appendix. The analyses were carried out after approval by the local Ethics Committee according to the guidelines of the Declaration of Helsinki and good clinical practice. Informed consent was obtained from the patients. Live-cell imaging kineticsCells were seeded in eight-well microscope chambers (Ibidi) that were coated with fibrinogen or collagen IV, at a concentration of 30,000 and 60,000 cells per well and imaged as previously described. 13 Retroviral transductionRetroviral particles were produced using Phoenix alpha packaging cells and inducible cell lines were established according to the manufacturer's instructions. Detailed information concerning oligonucleotide sequences and the backbones used is provided in the Online Supplementary Appendix. In vitro ubiquitinationThe APC/C was immunopurified from DG-75 and Kasumi-1 cells using an anti-Cdc27 antibody (Sigma-Aldrich) and Protein Gagarose. Ubiquitination reactions using precipitated APC/C were performed in the presence of in vitro transcribed/translated 35S-marked cyclin B as described in detail in the Online Supplementary Appendix. Western blot analysisWestern blotting was performed as described previously 13 using the antibodies specified in the Online Supplementary Appendix. Flow cytometryCell cycle distribution and BubR1 expression in single cells were determined using a FACSCalibur (Becton Dickinson). Microarray data and data processingMicroarray datasets were obtained from the open-access NIH Gene-Expression Omnibus (GEO) database. Datasets used in our analysis were GSE30029 18 and GSE13204.19 Data analysis and statistical analysisTIFF image stacks were analyzed using LSM Image Browser (v.2.80.1123) (Carl Zeiss). Calculations and statistics were done in Microsoft Excel 2002 and/or GraphPad Prism V5.03 (GraphPad Software Inc.). P values <0.05 were considered statistically significant. The statistical test used was an unpaired t-test (two-tailed) with a confidence interval of 95%. Results The mitotic checkpoint protein BubR1 is repressed in acute myeloid leukemiaTo address the expression levels of the regulatory proteins BubR1, ...

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Section: Discussionmentioning

confidence: 99%

BubR1 is frequently repressed in acute myeloid leukemia and its re-expression sensitizes cells to antimitotic therapy

Schnerch¹,

Schmidts²,

Follo³

et al. 2013

Haematologica

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“…Oral vinorelbine (VRL) has shown bioavailability of 40%, which is practically not influenced by food or age, moderate interpatient variability, and linear pharmacokinetics (17)(18)(19)(20). Its metabolism has been elucidated and only 4-O-deacetylvinorelbine (DVRL) has been found active (21)(22)(23)(24).…”

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confidence: 99%

“…Its metabolism has been elucidated and only 4-O-deacetylvinorelbine (DVRL) has been found active (21)(22)(23)(24). Both VRL and DVRL are mostly eliminated via the bile, and only limited amounts are excreted in urine (20,25). The elimination half-life of VRL is ∼40 hours and 168 hours for DVRL (20,25,26).…”

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confidence: 99%

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Dose-Ranging Study of Metronomic Oral Vinorelbine in Patients with Advanced Refractory Cancer

Briasoulis

Pappas

Puozzo

et al. 2009

Clinical Cancer Research

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Aim: To determine the safe dose range and pharmacokinetics of metronomic oral vinorelbine and obtain preliminary data on biomarkers and efficacy in patients with advanced cancer. Methods: Successive cohorts of patients received escalated doses of oral vinorelbine given thrice a week until disease progression, unacceptable toxicity (UT), or consent withdrawal. UT was any grade 4 toxicity, or grade 2 or 3 toxicity that would result to longer than 2-week break during the first 2 months of treatment. Blood samples were collected for pharmacokinetics and quantification of angiogenesis regulatory proteins. Results: Sixty-two patients (median age, 60 years) enrolled at six dose levels from 20 to 70 mg and received treatment for median 12.25 weeks (range, 2-216+). Unacceptable toxicity occurred in two of six patients treated at 60 mg (leucopenia grade 4 and epistaxis grade 2) and in one at 70 mg (leucopenia grade 2). The upper metronomic dose was 50 mg. Objective antitumor response documented in eight cases and 32% of patients experienced disease stability for minimum 6 months. Three responders (renal cancer, medullary thyroid carcinoma, and Kaposi sarcoma) received nonstop treatment for over 3 years without overt toxicity. Low pretreatment levels of circulating interleukin-8, vascular endothelial growth factor, and basic fibroblast growth factor were found predictors of efficacy. Steady-state concentrations of vinorelbine and its active metabolite ranged from 0.5 to 1.5 ng/mL. Conclusions: Metronomic administration of oral vinorelbine is feasible at doses up to 50 mg thrice a week and can yield sustainable antitumor activity without overt toxicity, probably through antiangiogenic mechanism. Further clinical investigation is warranted. (Clin Cancer Res 2009;15(20):6454-61)

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“…The oral formulation of vinorelbine is particularly interesting because it is rapidly absorbed, has an elimination half-life of 40 h, is highly bound to platelets, has a hepatic metabolism and an absolute bioavailability of 40%, being similar to that of the parental drug [7]. Pharmacologic exposure of 80 and 60 mg/m 2 of oral vinorelbine per week is equivalent to that of the standard doses of 30 and 25 mg/m 2 , respectively, administered intravenously [8], whereas food has no effect on its pharmacokinetics [9]. …”

Section: Introductionmentioning

confidence: 99%

A Dose Escalation Study of Biweekly Oral Vinorelbine and Gemcitabine in Patients with Solid Tumors

Karampeazis

Vamvakas²,

Agelaki³

et al. 2006

Oncology

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Purpose: To determine the maximum tolerated doses (MTDs) and the dose-limiting toxicities of a biweekly administration of oral vinorelbine and gemcitabine in patients with advanced solid tumors. Patients and Methods: Twenty-eight patients with advanced stage solid tumors were enrolled, and 12 (42.9%) of them were chemotherapy naive. Escalating doses of vinorelbine (50–70 mg/m² per os) and gemcitabine (800–1,000 mg/m² as a 30-min intravenous infusion) were administered on days 1 and 15 in 4-week cycles. Results: MTDs were reached at 70 mg/m² p.o. for vinorelbine and 900 mg/m² for gemcitabine. Grade 4 neutropenia, febrile neutropenia, grade 4 nausea/vomiting and treatment delay due to grade 3 neutropenia were the dose-limiting events during the first cycle of chemotherapy. A total of 94 chemotherapy cycles were administered with only one episode of febrile neutropenia and no toxic deaths. Severe (grade 3–4) neutropenia occurred in 10% of cycles while non-hematological toxicity was mild with grade 2–3 asthenia occurring in 17 (18%) cycles. Objective responses were achieved in patients with prostate and non-small cell lung cancer. Conclusions: The combination of biweekly oral vinorelbine (70 mg/m²) and gemcitabine (900 mg/m²) is a well-tolerated regimen with promising results in patients with advanced solid tumors.

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Oral versus intravenous vinorelbine: clinical safety profile

Cited by 65 publications

References 56 publications

BubR1 is frequently repressed in acute myeloid leukemia and its re-expression sensitizes cells to antimitotic therapy

BubR1 is frequently repressed in acute myeloid leukemia and its re-expression sensitizes cells to antimitotic therapy

Dose-Ranging Study of Metronomic Oral Vinorelbine in Patients with Advanced Refractory Cancer

A Dose Escalation Study of Biweekly Oral Vinorelbine and Gemcitabine in Patients with Solid Tumors

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