Pharmacokinetics and the bystander effect in CD::UPRT/5-FC bi-gene therapy of glioma

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SHI Dezhi HU Weixing LI Lixin CHEN Gong WEI Dong GU Peiyuan Department of NeurosurgeryFirst Affiliated Hospital of Nanjing Medical UniversityNanjingJiangsu China [210029 ]
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R686 [筋腱、韧带、滑囊疾病及损伤];
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1002 ; 100210 ;
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Background Cytosine deaminase (CD) converts 5-fluorocytosine (5-FC) to 5-fluorouracil (5-FU) in CD/5-FC genetherapy,5-FU will be mostly converted into nontoxic β-alanine without uracil phosphoribosyltransferase (UPRT).UPRTcatalyzes the conversion of 5-FU to 5-fluorouridine monophosphate,which directly kills CD::UPRT-expressing cells andsurrounding cells via the bystander effect.But the pharmacokinetics and the bystander effect of CD::UPRT/5-FC has notbeen verified in vivo and in vitro.Before the CD::UPRT/5-FC bi-gene therapy system is used in clinical trial,it is essentialto monitor the transgene expression and function in vivo.Thus,we developed a preclinical tumor model to investigate thefeasibility of usingF-magnetic resonance spectroscopy (F-MRS) and optical imaging to measure non-invasive CDand UPRT expression and its bystander effect.Methods C6 and C6-CD::UPRT cells were cultured with 5-FC.The medium,cells and their mixture were analyzed by19F-MRS.Rats with intracranial xenografted encephalic C6-CD::UPRT glioma were injected intraperitoneally with 5-FCand theirF-MRS spectra recorded.Then the pharmacokinetics of 5-FC was proved.Mixtures of C6 and C6-CD::UPRTcells at different ratios were cultured with 5-FC and the cytotoxic efficacy and survival rate of cells recorded.To determinethe mechanism of the bystander effect,the culture media from cell comprising 25% and 75% C6-CD::UPRT cells wereexamined byF-MRS.A comparative study of mean was performed using analysis of variance (ANOVA).ResultsF-MRS on samples from C6-CD::UPRT cells cultured with 5-FC showed three broad resonance signalscorresponding to 5-FC,5-FU and fluorinated nucleotides (F-Nuctd).For the C6 mixture,only the 5-FC peak was detected.Invivo serialF-MRS spectra showed a strong 5-FC peak and a weak 5-FU peak at 20 minutes after 5-FC injection.The5-FU concentration reached a maximum at about 50 minutes.The F-Nuctd signal appeared after about 1 hour,reached amaximum at around 160 minutes,and was detectable for several hours.At a 10% ratio of C6-CD::UPRT cells,thesurvival rate was (79.55±0.88)% (P <0.01).As the C6-CD::UPRT ratio increased,the survival rate of the cells decreased.F-MRS showed that the signals for 5-FU and F-Nuctd in the culture medium increased as the ratio of C6-CD::UPRT inthe mixture increased.ConclusionsF-MRS studies indicated that C6-CD::UPRT cells could effectively express CD and UPRT enzymes.The CD::UPRT/5-FC system showed an obvious bystander effect.This study demonstrated that CD::UPRT/5-FC genetherapy is suitable for 5-FC to F-Nuctd metabolism; andF-MRS can monitor transferred CD::UPRT gene expressionand catalysis of substrates noninvasively,dynamically and quantitatively.
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页码:1267 / 1272
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