Ursodeoxycholic Acid May Inhibit Deoxycholic Acid-Induced Apoptosis by Modulating Mitochondrial Transmembrane Potential and Reactive Oxygen Species Production

Rodrigues, C.M.P.; Gao, Fan; Wong, Phillip; Kren, Betsy T.; Steer, Clifford J.

doi:10.1007/bf03401914

Cited by 281 publications

(271 citation statements)

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“…[107][108][109] UDCA treatment dilutes the concentration of DCA, and is thought to modulate the membrane and inflammatory effects of secondary bile acids on the colonic mucosa by increasing the hydrophilicity of the colonic bile acid milieu, and suppressing cell-signaling pathways activated by DCA. 110,111 Problematically, bile acid 7a-dehydroxylating bacteria, including Clostridium scindens and C. hiranonas are capable of converting UDCA to LCA through bile acid 7b-dehydroxylation. 8 Studies have shown that LCA is toxic, and causes DNA damage in bacteria 112 and colonocytes.…”

Section: Inactivation Of Ursodeoxycholic Acid By 7b-dehydroxylationmentioning

confidence: 99%

Consequences of bile salt biotransformations by intestinal bacteria

et al. 2016

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Section: Inactivation Of Ursodeoxycholic Acid By 7b-dehydroxylationmentioning

confidence: 99%

Consequences of bile salt biotransformations by intestinal bacteria

et al. 2016

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“…11 In fact, UDCA appears to regulate apoptosis in both hepatic and nonhepatic cells by preventing mitochondrial depolarization and reactive oxygen species production. 10,13 Interestingly, the ability of UDCA to inhibit apoptosis appears to be independent of the inducing agent and its pathway, suggesting a common antiapoptotic mechanism(s). In particular, while the pathway to execution may be more direct with DCA, the apoptosis from TGF-b1 and okadaic acid are equally sensitive to the inhibitory effects of UDCA.…”

Section: Discussionmentioning

confidence: 99%

“…In vivo DCA feeding was associated with a 4.5-fold increase in mitochondrial-associated Bax protein levels, while combination feeding with UDCA significantly inhibited these changes. 13 Like Bcl-2, UDCA appears to modulate Bax-induced events at several levels, including prevention of Bax redistribution, inhibition of cytochrome c release, and modulation of cytochrome cmediated downstream events such as DEVD-specific caspase activity and PARP cleavage. It remains to be determined whether other factors, such as Bid-induced conformational change of Bax and cytochrome c release, 64 are in some way modulated by UDCA.…”

Section: Discussionmentioning

confidence: 99%

“…The effect was observed for a variety of agents acting through different apoptotic pathways involving mitochondrial membrane perturbation. 10,13 It is widely recognized that alterations in mitochondrial function, and particularly the MPT, play a key role during apoptosis in many cell types. In fact, the loss of mitochondrial transmembrane potential (Dc m ), release of caspase activators and participation of pro-and antiapoptotic Bcl-2 family proteins appear to be critical events during apoptosis.…”

Section: Introductionmentioning

confidence: 99%

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Ursodeoxycholic acid prevents cytochrome c release in apoptosis by inhibiting mitochondrial membrane depolarization and channel formation

et al. 1999

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The hydrophilic bile salt ursodeoxycholic acid (UDCA) is a potent inhibitor of apoptosis. In this paper, we further characterize the mechanism by which UDCA inhibits apoptosis induced by deoxycholic acid, okadaic acid and transforming growth factor b1 in primary rat hepatocytes. Our data indicate that coincubation of cells with UDCA and each of the apoptosis-inducing agents was associated with an approximately 80% inhibition of nuclear fragmentation (P50.001). Moreover, UDCA prevented mitochondrial release of cytochrome c into the cytoplasm by 70 ± 75% (P50.001), thereby, inhibiting subsequent activation of DEVD-specific caspases and cleavage of poly(ADP-ribose) polymerase. Each of the apoptosis-inducing agents decreased mitochondrial transmembrane potential and increased mitochondrial-associated Bax protein levels. Coincubation with UDCA was associated with significant inhibition of these mitochondrial membrane alterations. The results suggest that the mechanism by which UDCA inhibits apoptosis involves an interplay of events in which both depolarization and channel-forming activity of the mitochondrial membrane are inhibited.

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“…26 Extracts were prepared from nuclei and highly purified mitochondria isolated from rat liver, and the authenticity and purity of the extracts established by Western blot, enzymatic activity and electron microscopy. [28][29][30] Using this PCR-independent bacterial read-out system and extracts derived from rat liver, we have observed a chimeraplast-specific and mitochondrial protein extract dose-dependent growth of dual resistant colonies, ranging from 0.003 ± 0.002% to 0.05 ± 0.002%. This rate of repair in vitro did not differ significantly from that observed in parallel reactions using rat liver nuclear extract.…”

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confidence: 99%

Modification of hepatic genomic DNA using RNA/DNA oligonucleotides

Kren¹,

Chen

Felsheim

et al. 2002

Gene Ther

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Inherited metabolic diseases impose a significant worldwide burden both financially and socially. Although there have been advances in treating these disorders, alternative therapeutic approaches are being developed to correct the responsible genetic defects. Gene augmentation using viral vectors and transgene expression to replace an absent or defective protein has shown limited success in treating a variety of genetic disorders. In fact, the mechanisms by which cells and organisms protect against viral infections have presented significant barriers for long-term stable expression of the introduced transgene. In part, due to the disadvantages of using biological vectors, a variety of different approaches for nonviral gene delivery have been developed. 1 In particular, targeting of nonviral delivery systems to specific tissues by receptor/ligand interactions has been exploited for in vivo gene transfer. 2 By targeting the asialoglycoprotein receptor (ASGPR), gene delivery to hepatocytes has been significantly improved both in vitro 3 and in vivo. 4,5 Thus, we have focused on using nonviral approaches to correct the genetic defect in hepatocytes using galactosylated compounds attached directly to polycations, or incorporated in liposomes. 6 The strategy of in situ genomic repair using chimeric RNA/DNA molecules (chimeraplasts) developed from studies investigating molecular aspects of DNA repair. It became apparent that there was a significant increase in pairing efficiency between an oligonucleotide Յ50 bases and a genomic DNA target if RNA replaced DNA in a portion of the targeting oligonucleotide. 7,8 The original chimeric 68-mer design incorporated 10 2'-O-methylated RNA residues flanking each side of a 5 bp stretch of DNA, poly-T hairpin loops, a 3' GC clamp and a complementary all-DNA strand resulting in a stable, nucleaseresistant duplex molecule. The 25 bp homology segment between the chimeraplast and its genomic target is constructed such that it includes one mismatch with the DNA sequence of the gene. This engineered mismatch permits the directed alteration of the genomic target using the chimeraplast as a template for the intended correction of target sequence. It is postulated that the 'mismatched' chimeraplast complexes with the genomic DNA and creates the illusion of a genetic mutation leading to the recruitment of endogenous repair functions. 9,10 This novel approach of gene repair, based on in vitro experimental evidence, was shown by Yoon et al 11 and Cole-Strauss et al 12 to be capable of introducing targeted single base conversions in episomal and genomic DNA in cultured cells. We then reported that the chimeraplast

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Ursodeoxycholic Acid May Inhibit Deoxycholic Acid-Induced Apoptosis by Modulating Mitochondrial Transmembrane Potential and Reactive Oxygen Species Production

Cited by 281 publications

References 46 publications

Consequences of bile salt biotransformations by intestinal bacteria

Consequences of bile salt biotransformations by intestinal bacteria

Ursodeoxycholic acid prevents cytochrome c release in apoptosis by inhibiting mitochondrial membrane depolarization and channel formation

Modification of hepatic genomic DNA using RNA/DNA oligonucleotides

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