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- Publisher Website: 10.1007/BF01000240
- Scopus: eid_2-s2.0-0023254202
- PMID: 2439934
- WOS: WOS:A1987H384000010
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Article: The dynamics of cGMP metabolism in neuroblastoma N1E-115 cells determined by 18O labeling of guanine nucleotide α-phosphoryls
| Title | The dynamics of cGMP metabolism in neuroblastoma N1E-115 cells determined by 18O labeling of guanine nucleotide α-phosphoryls |
|---|---|
| Authors | |
| Keywords | Chemicals And Cas Registry Numbers |
| Issue Date | 1987 |
| Publisher | Springer New York LLC. The Journal's web site is located at http://springerlink.metapress.com/openurl.asp?genre=journal&issn=0364-3190 |
| Citation | Neurochemical Research, 1987, v. 12 n. 6, p. 551-560 How to Cite? |
| Abstract | The rates of phosphodiesterase-promoted hydrolysis of cGMP and cAMP have been measured in intact neuroblastoma N1E-115 cells by determining of 18O incorporation from 18O-water into the α-phosphoryls of guanine and adenine nucleotides. The basal rate of guanine nucleotide α-phosphoryl labeling ranged from 180 to 244 pmol·mg protein-1·min-1. Sodium nitroprusside (SNP) caused a sustained 3.4-fold increase in this 18O-labeling rate in conjunction with 28- and 50-fold increases in cellular cGMP concentration at 3 and 6 min, respectively. This 18O-labeling rate (795 pmol·mg protein-1·min-1) corresponded with the sum of the low (1.7 μM) and high (34 μM) K(m) phosphodiesterase activities assayable in cell lysates which exhibited a combined maximum velocity of 808 pmol·mg protein-1·min-1 to which the high K(m) species contributed 84%. This information and the characteristics of the profile of 18O-labeled molecular species indicate that cGMP metabolism was restricted to a very discrete cellular compartment(s) of approximately 12% of the cell volume. Carbachol (1 mM) produced a transient increase (6-fold) in cellular cGMP concentration and a transient increase (90%) in the rate of 18O labeling of α-GTP during the first minute of treatment which translates into 30 additional cellular pools of cGMP hydrolyzed in this period. IBMX (1 mM) produced a relatively rapid increase in cellular cGMP (3- to 5-fold) and cAMP (2-fold) concentrations and a delayed inhibition of 18O labeling of guanine and adenine nucleotide α-phosphoryls without further elevation of cyclic nucleotide levels. These results indicate that besides inhibiting cyclic nucleotide hydrolysis, IBMX also imparts a time-dependent inhibitory influence on the generation of cyclic nucleotides. The data obtained show that measurement of 18O labeling of guanine and adenine nucleotide α-phosphoryls combined with measurements of cyclic nucleotide steady state levels provides a means to assess the rates of cyclic nucleotide synthesis and hydrolysis within intact cells and to identify the site(s) of action of agents that alter cellular cyclic nucleotide metabolism. |
| Persistent Identifier | http://hdl.handle.net/10722/132592 |
| ISSN | 2021 Impact Factor: 4.414 2020 SCImago Journal Rankings: 1.102 |
| ISI Accession Number ID |
| DC Field | Value | Language |
|---|---|---|
| dc.contributor.author | Graeff, RM | en_HK |
| dc.contributor.author | Walseth, TF | en_HK |
| dc.contributor.author | Goldberg, ND | en_HK |
| dc.date.accessioned | 2011-03-28T09:26:35Z | - |
| dc.date.available | 2011-03-28T09:26:35Z | - |
| dc.date.issued | 1987 | en_HK |
| dc.identifier.citation | Neurochemical Research, 1987, v. 12 n. 6, p. 551-560 | en_HK |
| dc.identifier.issn | 0364-3190 | en_HK |
| dc.identifier.uri | http://hdl.handle.net/10722/132592 | - |
| dc.description.abstract | The rates of phosphodiesterase-promoted hydrolysis of cGMP and cAMP have been measured in intact neuroblastoma N1E-115 cells by determining of 18O incorporation from 18O-water into the α-phosphoryls of guanine and adenine nucleotides. The basal rate of guanine nucleotide α-phosphoryl labeling ranged from 180 to 244 pmol·mg protein-1·min-1. Sodium nitroprusside (SNP) caused a sustained 3.4-fold increase in this 18O-labeling rate in conjunction with 28- and 50-fold increases in cellular cGMP concentration at 3 and 6 min, respectively. This 18O-labeling rate (795 pmol·mg protein-1·min-1) corresponded with the sum of the low (1.7 μM) and high (34 μM) K(m) phosphodiesterase activities assayable in cell lysates which exhibited a combined maximum velocity of 808 pmol·mg protein-1·min-1 to which the high K(m) species contributed 84%. This information and the characteristics of the profile of 18O-labeled molecular species indicate that cGMP metabolism was restricted to a very discrete cellular compartment(s) of approximately 12% of the cell volume. Carbachol (1 mM) produced a transient increase (6-fold) in cellular cGMP concentration and a transient increase (90%) in the rate of 18O labeling of α-GTP during the first minute of treatment which translates into 30 additional cellular pools of cGMP hydrolyzed in this period. IBMX (1 mM) produced a relatively rapid increase in cellular cGMP (3- to 5-fold) and cAMP (2-fold) concentrations and a delayed inhibition of 18O labeling of guanine and adenine nucleotide α-phosphoryls without further elevation of cyclic nucleotide levels. These results indicate that besides inhibiting cyclic nucleotide hydrolysis, IBMX also imparts a time-dependent inhibitory influence on the generation of cyclic nucleotides. The data obtained show that measurement of 18O labeling of guanine and adenine nucleotide α-phosphoryls combined with measurements of cyclic nucleotide steady state levels provides a means to assess the rates of cyclic nucleotide synthesis and hydrolysis within intact cells and to identify the site(s) of action of agents that alter cellular cyclic nucleotide metabolism. | en_HK |
| dc.language | eng | en_US |
| dc.publisher | Springer New York LLC. The Journal's web site is located at http://springerlink.metapress.com/openurl.asp?genre=journal&issn=0364-3190 | en_HK |
| dc.relation.ispartof | Neurochemical Research | en_HK |
| dc.subject | Chemicals And Cas Registry Numbers | en_US |
| dc.title | The dynamics of cGMP metabolism in neuroblastoma N1E-115 cells determined by 18O labeling of guanine nucleotide α-phosphoryls | en_HK |
| dc.type | Article | en_HK |
| dc.identifier.email | Graeff, RM: graeffr@hku.hk | en_HK |
| dc.identifier.authority | Graeff, RM=rp01464 | en_HK |
| dc.description.nature | link_to_subscribed_fulltext | en_US |
| dc.identifier.doi | 10.1007/BF01000240 | - |
| dc.identifier.pmid | 2439934 | - |
| dc.identifier.scopus | eid_2-s2.0-0023254202 | en_HK |
| dc.identifier.volume | 12 | en_HK |
| dc.identifier.issue | 6 | en_HK |
| dc.identifier.spage | 551 | en_HK |
| dc.identifier.epage | 560 | en_HK |
| dc.identifier.isi | WOS:A1987H384000010 | - |
| dc.publisher.place | United States | en_HK |
| dc.identifier.scopusauthorid | Graeff, RM=7003614053 | en_HK |
| dc.identifier.scopusauthorid | Walseth, TF=7005424273 | en_HK |
| dc.identifier.scopusauthorid | Goldberg, ND=23085828700 | en_HK |
| dc.identifier.issnl | 0364-3190 | - |