Cellular Sensitization to m-Diamminedichloroplatinum(II) by Novel Analogues of the Protein Kinase C Activator Lyngbyatoxin A

Alakananda Basu; Alan P. Kozikowski; Kazuo Sato; John S. Lazo

Cellular Sensitization to m-Diamminedichloroplatinum(II) by Novel Analogues of the Protein Kinase C Activator Lyngbyatoxin A

Alakananda Basu, Alan P. Kozikowski, Kazuo Sato, John S. Lazo

Research output: Contribution to journal › Article › peer-review

Abstract

Protein kinase C (PKC) has been implicated in enhancing cellularsensitivity to m-diamminedichloroplatinum(II) (CP). We have synthesized a series of novel analogues of lyngbyatoxin A (7-linalylindolactamV), a natural tumor promoter and a potent activator of PKC, andinvestigated the effects of these synthetic compounds on PKC activityand the antiproliferative activity of CP. Lyngbyatoxin A was as effectiveas phorbol esters, such as 12-0-tetradecanoylphorboM3-acetate, in enhancing the sensitivity of HeLa cells to CP. A 24-h pretreatment of HeLacells with 1 to 100 IIM lyngbyatoxin A caused an approximately 9-foldsensitization to CP. All analogues of lyngbyatoxin A that retained thelactam ring portion of the molecule but contained different hydrophobicsubstituents at C-7 including indolactam V (ILV), fert-butyl-ILV, or nhexyl-ILV increased cellular sensitivity to CP in a concentration-dependent manner. Maximum cellular sensitization to CP (9-fold) was seen with10 nM n-hexyl or ferr-butyl compounds, and ILV devoid of any C-7substitution required higher concentrations (1 n\\) for equivalent sensitization. The ability of lyngbyatoxin A analogues to sensitize cells to CPcorrelated directly with their ability to activate PKC in vitro. Syntheticanalogues that lacked the lactam ring structure neither activated PKCnor sensitized cells to CP. The C-9 epi analogue of n-hexyl-ILV was lesseffective than the corresponding natural stereoisomer in activating PKCas well as sensitizing cells to CP. Exposure of HeLa cells to 100 nMlyngbyatoxin A for 24 h caused a substantial decrease in cellular PKCactivity to 20% of the untreated control value, but a similar treatment of cells with n-hexyl- or fert-butyl-ILV led to only a 25% reduction in PKCactivity. Concentrations of ILV (e.g. 1 MM)that sensitized HeLa cells toCP caused no down-regulation of PKC. Thus, on the basis of results withthese novel lyngbyatoxin A analogues, we conclude that activation butnot down-regulation of PKC is necessary for sensitization of HeLa cellsto CP.

Original language	English (US)
Pages (from-to)	2511-2514
Number of pages	4
Journal	Cancer Research
Volume	51
Issue number	10
State	Published - May 1991
Externally published	Yes

ASJC Scopus subject areas

Oncology
Cancer Research

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title = "Cellular Sensitization to m-Diamminedichloroplatinum(II) by Novel Analogues of the Protein Kinase C Activator Lyngbyatoxin A",

abstract = "Protein kinase C (PKC) has been implicated in enhancing cellularsensitivity to m-diamminedichloroplatinum(II) (CP). We have synthesized a series of novel analogues of lyngbyatoxin A (7-linalylindolactamV), a natural tumor promoter and a potent activator of PKC, andinvestigated the effects of these synthetic compounds on PKC activityand the antiproliferative activity of CP. Lyngbyatoxin A was as effectiveas phorbol esters, such as 12-0-tetradecanoylphorboM3-acetate, in enhancing the sensitivity of HeLa cells to CP. A 24-h pretreatment of HeLacells with 1 to 100 IIM lyngbyatoxin A caused an approximately 9-foldsensitization to CP. All analogues of lyngbyatoxin A that retained thelactam ring portion of the molecule but contained different hydrophobicsubstituents at C-7 including indolactam V (ILV), fert-butyl-ILV, or nhexyl-ILV increased cellular sensitivity to CP in a concentration-dependent manner. Maximum cellular sensitization to CP (9-fold) was seen with10 nM n-hexyl or ferr-butyl compounds, and ILV devoid of any C-7substitution required higher concentrations (1 n\\) for equivalent sensitization. The ability of lyngbyatoxin A analogues to sensitize cells to CPcorrelated directly with their ability to activate PKC in vitro. Syntheticanalogues that lacked the lactam ring structure neither activated PKCnor sensitized cells to CP. The C-9 epi analogue of n-hexyl-ILV was lesseffective than the corresponding natural stereoisomer in activating PKCas well as sensitizing cells to CP. Exposure of HeLa cells to 100 nMlyngbyatoxin A for 24 h caused a substantial decrease in cellular PKCactivity to 20% of the untreated control value, but a similar treatment of cells with n-hexyl- or fert-butyl-ILV led to only a 25% reduction in PKCactivity. Concentrations of ILV (e.g. 1 MM)that sensitized HeLa cells toCP caused no down-regulation of PKC. Thus, on the basis of results withthese novel lyngbyatoxin A analogues, we conclude that activation butnot down-regulation of PKC is necessary for sensitization of HeLa cellsto CP.",

author = "Alakananda Basu and Kozikowski, {Alan P.} and Kazuo Sato and Lazo, {John S.}",

year = "1991",

month = may,

language = "English (US)",

volume = "51",

pages = "2511--2514",

journal = "Cancer Research",

issn = "0008-5472",

publisher = "American Association for Cancer Research Inc.",

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TY - JOUR

T1 - Cellular Sensitization to m-Diamminedichloroplatinum(II) by Novel Analogues of the Protein Kinase C Activator Lyngbyatoxin A

AU - Basu, Alakananda

AU - Kozikowski, Alan P.

AU - Sato, Kazuo

AU - Lazo, John S.

PY - 1991/5

Y1 - 1991/5

N2 - Protein kinase C (PKC) has been implicated in enhancing cellularsensitivity to m-diamminedichloroplatinum(II) (CP). We have synthesized a series of novel analogues of lyngbyatoxin A (7-linalylindolactamV), a natural tumor promoter and a potent activator of PKC, andinvestigated the effects of these synthetic compounds on PKC activityand the antiproliferative activity of CP. Lyngbyatoxin A was as effectiveas phorbol esters, such as 12-0-tetradecanoylphorboM3-acetate, in enhancing the sensitivity of HeLa cells to CP. A 24-h pretreatment of HeLacells with 1 to 100 IIM lyngbyatoxin A caused an approximately 9-foldsensitization to CP. All analogues of lyngbyatoxin A that retained thelactam ring portion of the molecule but contained different hydrophobicsubstituents at C-7 including indolactam V (ILV), fert-butyl-ILV, or nhexyl-ILV increased cellular sensitivity to CP in a concentration-dependent manner. Maximum cellular sensitization to CP (9-fold) was seen with10 nM n-hexyl or ferr-butyl compounds, and ILV devoid of any C-7substitution required higher concentrations (1 n\\) for equivalent sensitization. The ability of lyngbyatoxin A analogues to sensitize cells to CPcorrelated directly with their ability to activate PKC in vitro. Syntheticanalogues that lacked the lactam ring structure neither activated PKCnor sensitized cells to CP. The C-9 epi analogue of n-hexyl-ILV was lesseffective than the corresponding natural stereoisomer in activating PKCas well as sensitizing cells to CP. Exposure of HeLa cells to 100 nMlyngbyatoxin A for 24 h caused a substantial decrease in cellular PKCactivity to 20% of the untreated control value, but a similar treatment of cells with n-hexyl- or fert-butyl-ILV led to only a 25% reduction in PKCactivity. Concentrations of ILV (e.g. 1 MM)that sensitized HeLa cells toCP caused no down-regulation of PKC. Thus, on the basis of results withthese novel lyngbyatoxin A analogues, we conclude that activation butnot down-regulation of PKC is necessary for sensitization of HeLa cellsto CP.

AB - Protein kinase C (PKC) has been implicated in enhancing cellularsensitivity to m-diamminedichloroplatinum(II) (CP). We have synthesized a series of novel analogues of lyngbyatoxin A (7-linalylindolactamV), a natural tumor promoter and a potent activator of PKC, andinvestigated the effects of these synthetic compounds on PKC activityand the antiproliferative activity of CP. Lyngbyatoxin A was as effectiveas phorbol esters, such as 12-0-tetradecanoylphorboM3-acetate, in enhancing the sensitivity of HeLa cells to CP. A 24-h pretreatment of HeLacells with 1 to 100 IIM lyngbyatoxin A caused an approximately 9-foldsensitization to CP. All analogues of lyngbyatoxin A that retained thelactam ring portion of the molecule but contained different hydrophobicsubstituents at C-7 including indolactam V (ILV), fert-butyl-ILV, or nhexyl-ILV increased cellular sensitivity to CP in a concentration-dependent manner. Maximum cellular sensitization to CP (9-fold) was seen with10 nM n-hexyl or ferr-butyl compounds, and ILV devoid of any C-7substitution required higher concentrations (1 n\\) for equivalent sensitization. The ability of lyngbyatoxin A analogues to sensitize cells to CPcorrelated directly with their ability to activate PKC in vitro. Syntheticanalogues that lacked the lactam ring structure neither activated PKCnor sensitized cells to CP. The C-9 epi analogue of n-hexyl-ILV was lesseffective than the corresponding natural stereoisomer in activating PKCas well as sensitizing cells to CP. Exposure of HeLa cells to 100 nMlyngbyatoxin A for 24 h caused a substantial decrease in cellular PKCactivity to 20% of the untreated control value, but a similar treatment of cells with n-hexyl- or fert-butyl-ILV led to only a 25% reduction in PKCactivity. Concentrations of ILV (e.g. 1 MM)that sensitized HeLa cells toCP caused no down-regulation of PKC. Thus, on the basis of results withthese novel lyngbyatoxin A analogues, we conclude that activation butnot down-regulation of PKC is necessary for sensitization of HeLa cellsto CP.

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Cellular Sensitization to m-Diamminedichloroplatinum(II) by Novel Analogues of the Protein Kinase C Activator Lyngbyatoxin A

Abstract

ASJC Scopus subject areas

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