An investigation of the temporal induction of cytokine mRNAs in LPS-challenged thioglycollate-elicited murine peritoneal macrophages using the reverse transcription polymerase chain reaction
A comprehensive study to standardise interleukin (IL)-1 alpha, -1 beta, -6, -10, -12 and tumour necrosis factor alpha (TNF alpha) mRNA detection in murine peritoneal macrophages, using the reverse transcription polymerase chain reaction (RT-PCR) was carried out. Thioglycollate-elicited peritoneal ex...
Saved in:
| Published in | Inflammation research Vol. 46; no. 2; pp. 65 - 71 |
|---|---|
| Main Authors | , , |
| Format | Journal Article |
| Language | English |
| Published |
Switzerland
01.02.1997
|
| Subjects | |
| Online Access | Get full text |
| ISSN | 1023-3830 1420-908X |
| DOI | 10.1007/s000110050078 |
Cover
| Abstract | A comprehensive study to standardise interleukin (IL)-1 alpha, -1 beta, -6, -10, -12 and tumour necrosis factor alpha (TNF alpha) mRNA detection in murine peritoneal macrophages, using the reverse transcription polymerase chain reaction (RT-PCR) was carried out.
Thioglycollate-elicited peritoneal exudate cells were harvested from female BALB/c mice and the adherent macrophage fraction isolated for use.
Peritoneal macrophages (1 x 10(6)) were incubated in the presence or absence of lipopolysaccharide (LPS; at a final concentration of 1 microgram/ml) for 0, 1, 2, 3, 4, 5 and 24 h.
Culture supernatants and cells were harvested at each time point, the secreted cytokine protein levels quantified by sandwich immunoassays and the cytokine mRNA levels assessed by RT-PCR.
The IL-6 mRNA was not expressed in detectable amounts in the macrophages, unless challenged with LPS. TNF alpha, IL-1 alpha, IL-1 beta, IL-10 and IL-12 mRNAs were expressed in both stimulated and unstimulated macrophages. The levels of the PCR products and thus mRNAs of all the cytokines increased with LPS stimulation, maximal levels being achieved 3 to 5 h post stimulation.
RT-PCR produced consistent results, indicating that this technique could be used to investigate the effect of biological mediators and novel pharmacological agents on cytokine mRNA levels in macrophages. |
|---|---|
| AbstractList | A comprehensive study to standardise interleukin (IL)-1 alpha , -1 beta , -6, -10, -12 and tumour necrosis factor alpha (TNF alpha ) mRNA detection in murine peritoneal macrophages, using the reverse transcription polymerase chain reaction (RT-PCR) was carried out. Thioglycollate-elicited peritoneal exudate cells were harvested from female BALB/c mice and the adherent macrophage fraction isolated for use. Peritoneal macrophages (1 x 10 super(6)) were incubated in the presence or absence of lipopolysaccharide (LPS; at a final concentration of 1 mu g/ml) for 0, 1, 2, 3, 4, 5 and 24 h. Culture supernatants and cells were harvested at each time point, the secreted cytokine protein levels quantified by sandwich immunoassays and the cytokine mRNA levels assessed by RT-PCR. The IL-6 mRNA was not expressed in detectable amounts in the macrophages, unless challenged with LPS. TNF alpha , IL-1 alpha , IL-1 beta , IL-10 and IL-12 mRNAs were expressed in both stimulated and unstimulated macrophages. The levels of the PCR products and thus mRNAs of all the cytokines increased with LPS stimulation, maximal levels being achieved 3 to 5 h post stimulation. RT-PCR produced consistent results, indicating that this technique could be used to investigate the effect of biological mediators and novel pharmacological agents on cytokine mRNA levels in macrophages. Objective and Design: A comprehensive study to standardise interleukin (IL)-1, -1, -6, -10, -12 and tumour necrosis factor alpha (TNF) mRNA detection in murine peritoneal macrophages, using the reverse transcription polymerase chain reaction (RT-PCR) was carried out. Subjects: Thioglycollate-elicited peritoneal exudate cells were harvested from female BALB/c mice and the adherent macrophage fraction isolated for use. Treatment: Peritoneal macrophages (110 super(6)) were incubated in the presence or absence of lipopolysaccharide (LPS; at a final concentration of 1 mu g/ml) for 0, 1, 2, 3, 4, 5 and 24h. Methods: Culture supernatants and cells were harvested at each time point, the secreted cytokine protein levels quantified by sandwich immunoassays and the cytokine mRNA levels assessed by RT-PCR. Results: The IL-6 mRNA was not expressed in detectable amounts in the macrophages, unless challenged with LPS. TNF, IL-1, IL-1, IL-10 and IL-12 mRNAs were expressed in both stimulated and unstimulated macrophages. The levels of the PCR products and thus mRNAs of all the cytokines increased with LPS stimulation, maximal levels being achieved 3 to 5h post stimulation. Conclusions: RT-PCR produced consistent results, indicating that this technique could be used to investigate the effect of biological mediators and novel pharmacological agents on cytokine mRNA levels in macrophages. A comprehensive study to standardise interleukin (IL)-1 alpha, -1 beta, -6, -10, -12 and tumour necrosis factor alpha (TNF alpha) mRNA detection in murine peritoneal macrophages, using the reverse transcription polymerase chain reaction (RT-PCR) was carried out. Thioglycollate-elicited peritoneal exudate cells were harvested from female BALB/c mice and the adherent macrophage fraction isolated for use. Peritoneal macrophages (1 x 10(6)) were incubated in the presence or absence of lipopolysaccharide (LPS; at a final concentration of 1 microgram/ml) for 0, 1, 2, 3, 4, 5 and 24 h. Culture supernatants and cells were harvested at each time point, the secreted cytokine protein levels quantified by sandwich immunoassays and the cytokine mRNA levels assessed by RT-PCR. The IL-6 mRNA was not expressed in detectable amounts in the macrophages, unless challenged with LPS. TNF alpha, IL-1 alpha, IL-1 beta, IL-10 and IL-12 mRNAs were expressed in both stimulated and unstimulated macrophages. The levels of the PCR products and thus mRNAs of all the cytokines increased with LPS stimulation, maximal levels being achieved 3 to 5 h post stimulation. RT-PCR produced consistent results, indicating that this technique could be used to investigate the effect of biological mediators and novel pharmacological agents on cytokine mRNA levels in macrophages. A comprehensive study to standardise interleukin (IL)-1 alpha, -1 beta, -6, -10, -12 and tumour necrosis factor alpha (TNF alpha) mRNA detection in murine peritoneal macrophages, using the reverse transcription polymerase chain reaction (RT-PCR) was carried out.OBJECTIVE AND DESIGNA comprehensive study to standardise interleukin (IL)-1 alpha, -1 beta, -6, -10, -12 and tumour necrosis factor alpha (TNF alpha) mRNA detection in murine peritoneal macrophages, using the reverse transcription polymerase chain reaction (RT-PCR) was carried out.Thioglycollate-elicited peritoneal exudate cells were harvested from female BALB/c mice and the adherent macrophage fraction isolated for use.SUBJECTSThioglycollate-elicited peritoneal exudate cells were harvested from female BALB/c mice and the adherent macrophage fraction isolated for use.Peritoneal macrophages (1 x 10(6)) were incubated in the presence or absence of lipopolysaccharide (LPS; at a final concentration of 1 microgram/ml) for 0, 1, 2, 3, 4, 5 and 24 h.TREATMENTPeritoneal macrophages (1 x 10(6)) were incubated in the presence or absence of lipopolysaccharide (LPS; at a final concentration of 1 microgram/ml) for 0, 1, 2, 3, 4, 5 and 24 h.Culture supernatants and cells were harvested at each time point, the secreted cytokine protein levels quantified by sandwich immunoassays and the cytokine mRNA levels assessed by RT-PCR.METHODSCulture supernatants and cells were harvested at each time point, the secreted cytokine protein levels quantified by sandwich immunoassays and the cytokine mRNA levels assessed by RT-PCR.The IL-6 mRNA was not expressed in detectable amounts in the macrophages, unless challenged with LPS. TNF alpha, IL-1 alpha, IL-1 beta, IL-10 and IL-12 mRNAs were expressed in both stimulated and unstimulated macrophages. The levels of the PCR products and thus mRNAs of all the cytokines increased with LPS stimulation, maximal levels being achieved 3 to 5 h post stimulation.RESULTSThe IL-6 mRNA was not expressed in detectable amounts in the macrophages, unless challenged with LPS. TNF alpha, IL-1 alpha, IL-1 beta, IL-10 and IL-12 mRNAs were expressed in both stimulated and unstimulated macrophages. The levels of the PCR products and thus mRNAs of all the cytokines increased with LPS stimulation, maximal levels being achieved 3 to 5 h post stimulation.RT-PCR produced consistent results, indicating that this technique could be used to investigate the effect of biological mediators and novel pharmacological agents on cytokine mRNA levels in macrophages.CONCLUSIONSRT-PCR produced consistent results, indicating that this technique could be used to investigate the effect of biological mediators and novel pharmacological agents on cytokine mRNA levels in macrophages. |
| Author | Cooper, K. L. Simpson, A. E. C. M. Tomkins, P. T. |
| Author_xml | – sequence: 1 givenname: A. E. C. M. surname: Simpson fullname: Simpson, A. E. C. M. – sequence: 2 givenname: P. T. surname: Tomkins fullname: Tomkins, P. T. – sequence: 3 givenname: K. L. surname: Cooper fullname: Cooper, K. L. |
| BackLink | https://www.ncbi.nlm.nih.gov/pubmed/9085146$$D View this record in MEDLINE/PubMed |
| BookMark | eNqFUktv1DAQtlBRaQtHjkg5IS4pfiR-HFcVL2nVVjwkbpGTnWQNjh3spNL-OX4b0-32QIXoxR77-775xjM-JUchBiDkJaPnjFL1NlNKGUY1HvQTcsIqTktD9fcjjCkXpdCCPiOnOf9ApuaaH5NjxGtWyRPyexUKF24gz26ws4uhiH0xb6GYYZxish7RzdLdI91ujj9dgGL8fLnKiBXr6y9lt7XeQxhgg1IXB7_rovd2hhK869yM9-OSbmUTJDdj_Zh3tF2K09YOkIsluzDsbRPcQMpon2zIXXLT3nmKfjdCsgigF7omsPuanpOnvfUZXhz2M_Lt_buvFx_L9dWHTxerddmJms8lLq21SloOloE0dVWD6AX0zHAwtFZM8FZWYKC3dcv6jayokn2lmOlbJag4I6_v8k4p_lqwW83ocgf4yABxyY3S2kipOBLf_JfIJFdG10byR3MySSk3WiLx1YG4tCNsmim50aZdcxgi4uIOx4bmnKBvsOf7YWIXnW8YbW5_SvPXT0FV-UB1n_ff_D8nTcMF |
| CitedBy_id | crossref_primary_10_1006_meth_1998_0645 crossref_primary_10_1021_jf1017719 crossref_primary_10_4049_jimmunol_1102595 crossref_primary_10_1016_j_cellimm_2005_12_002 crossref_primary_10_1067_mai_2001_114110 crossref_primary_10_1186_s12950_018_0193_8 crossref_primary_10_1016_j_ejphar_2004_11_035 crossref_primary_10_1038_nm814 crossref_primary_10_1074_jbc_M106114200 crossref_primary_10_4049_jimmunol_1501156 crossref_primary_10_1016_S0306_4522_02_00783_2 crossref_primary_10_4049_jimmunol_165_10_5906 crossref_primary_10_1086_526788 crossref_primary_10_1016_S0014_5793_00_01169_8 |
| ContentType | Journal Article |
| DBID | AAYXX CITATION CGR CUY CVF ECM EIF NPM 7T5 H94 7X8 |
| DOI | 10.1007/s000110050078 |
| DatabaseName | CrossRef Medline MEDLINE MEDLINE (Ovid) MEDLINE MEDLINE PubMed Immunology Abstracts AIDS and Cancer Research Abstracts MEDLINE - Academic |
| DatabaseTitle | CrossRef MEDLINE Medline Complete MEDLINE with Full Text PubMed MEDLINE (Ovid) AIDS and Cancer Research Abstracts Immunology Abstracts MEDLINE - Academic |
| DatabaseTitleList | AIDS and Cancer Research Abstracts AIDS and Cancer Research Abstracts MEDLINE MEDLINE - Academic |
| Database_xml | – sequence: 1 dbid: NPM name: PubMed url: https://proxy.k.utb.cz/login?url=http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed sourceTypes: Index Database – sequence: 2 dbid: EIF name: MEDLINE url: https://proxy.k.utb.cz/login?url=https://www.webofscience.com/wos/medline/basic-search sourceTypes: Index Database |
| DeliveryMethod | fulltext_linktorsrc |
| Discipline | Pharmacy, Therapeutics, & Pharmacology |
| EISSN | 1420-908X |
| EndPage | 71 |
| ExternalDocumentID | 9085146 10_1007_s000110050078 |
| Genre | Journal Article |
| GroupedDBID | --- -Y2 .55 .86 .GJ .VR 06C 06D 0R~ 0VY 199 1N0 203 29I 29~ 2J2 2JN 2JY 2KG 2KM 2LR 2P1 2VQ 2~H 30V 3O- 4.4 406 408 409 40D 40E 53G 5GY 5RE 5VS 67N 67Z 6NX 78A 7X7 88E 8AO 8FI 8FJ 8TC 8UJ 95- 95. 95~ 96X AABHQ AAHNG AAIAL AAJBT AAJKR AANXM AANZL AAPKM AARHV AARTL AASML AATVU AAWCG AAYIU AAYQN AAYTO AAYXX AAYZH ABAKF ABBBX ABBRH ABBXA ABDBE ABDZT ABECU ABFSG ABFTV ABHLI ABJNI ABJOX ABKCH ABKTR ABMNI ABMQK ABNWP ABOCM ABPLI ABQBU ABQSL ABSXP ABTEG ABTHY ABTKH ABTMW ABULA ABUWG ABWNU ABXPI ACAOD ACBXY ACGFS ACHSB ACHXU ACKNC ACMDZ ACMLO ACOKC ACOMO ACPRK ACSTC ACZOJ ADHIR ADHKG ADIMF ADKPE ADRFC ADTPH ADURQ ADYFF ADZKW AEBTG AEFQL AEGAL AEGNC AEJHL AEJRE AEKMD AEMSY AENEX AEOHA AEPYU AESKC AETLH AEVLU AEXYK AEZWR AFBBN AFDZB AFGCZ AFHIU AFKRA AFLOW AFRAH AFWTZ AFZKB AGAYW AGDGC AGGDS AGJBK AGMZJ AGQEE AGQMX AGRTI AGWIL AGWZB AGYKE AHBYD AHKAY AHMBA AHPBZ AHSBF AHWEU AHYZX AIAKS AIGIU AILAN AITGF AIXLP AJBLW AJRNO AJZVZ AKMHD ALIPV ALMA_UNASSIGNED_HOLDINGS ALWAN AMKLP AMXSW AMYLF AOCGG ARMRJ ATHPR AXYYD AYFIA AZFZN B-. BA0 BDATZ BENPR BSONS CCPQU CITATION CS3 CSCUP DDRTE DL5 DNIVK DPUIP DU5 EBLON EBS EIOEI EJD EN4 EPAXT ESBYG FEDTE FERAY FFXSO FIGPU FINBP FNLPD FRRFC FSGXE FWDCC FYUFA G-Y G-Z GGCAI GGRSB GJIRD GNWQR GQ7 GQ8 GXS HF~ HG5 HG6 HMCUK HMJXF HQYDN HRMNR HVGLF HZ~ IHE IJ- IKXTQ ITM IWAJR IXC IZIGR IZQ I~X I~Z J-C J0Z JBSCW JCJTX JZLTJ KDC KOV KPH LAS LLZTM M1P M4Y MA- N2Q NB0 NPVJJ NQJWS NU0 O9- O93 O9G O9I O9J OAM P19 P2P PF0 PHGZM PHGZT PSQYO PT4 PT5 QOK QOR QOS R89 R9I RHV RNI ROL RPX RRX RSV RZK S16 S27 S3A S3B SAP SBL SDH SDM SHX SISQX SJYHP SNE SNPRN SNX SOHCF SOJ SPISZ SRMVM SSLCW SSXJD STPWE SZN T13 TSG TSK TSV TUC U2A U9L UG4 UKHRP UOJIU UTJUX UZXMN VC2 VFIZW W23 W48 WH7 WJK WK8 X7M Y6R YLTOR Z45 ZGI ZMTXR ZOVNA ZXP ~EX ~KM -4W -56 -5G -BR -EM -~C 2.D 28- 3SX 3V. 5QI AAAVM AACDK AATNV AAUYE ABHQN ACDTI ADBBV ADINQ ADKNI ADYPR AEFIE AFEXP AFQWF AHAVH AIIXL BBWZM BGNMA BPHCQ BVXVI CAG CGR COF CUY CVF EBD ECM EIF GQ6 H13 KOW NDZJH NPM OVD PKN PQQKQ PROAC Q2X S1Z S26 S28 SBY SCLPG T16 TEORI WK6 Z7U Z7W Z82 Z87 Z8O Z8Q Z8V Z91 7T5 ABRTQ H94 PJZUB PPXIY PUEGO 7X8 |
| ID | FETCH-LOGICAL-c352t-352baa76a2ea1e69545e3f3ef192e9057132b64e9efa5b1fd64076f4719fb7303 |
| ISSN | 1023-3830 |
| IngestDate | Thu Sep 04 22:00:19 EDT 2025 Thu Sep 04 19:49:38 EDT 2025 Fri Sep 05 04:58:58 EDT 2025 Wed Feb 19 01:16:29 EST 2025 Thu Apr 24 23:08:03 EDT 2025 Tue Jul 01 01:43:33 EDT 2025 |
| IsPeerReviewed | true |
| IsScholarly | true |
| Issue | 2 |
| Language | English |
| License | http://www.springer.com/tdm |
| LinkModel | OpenURL |
| MergedId | FETCHMERGED-LOGICAL-c352t-352baa76a2ea1e69545e3f3ef192e9057132b64e9efa5b1fd64076f4719fb7303 |
| Notes | ObjectType-Article-2 SourceType-Scholarly Journals-1 ObjectType-Feature-1 content type line 23 ObjectType-Article-1 ObjectType-Feature-2 |
| PMID | 9085146 |
| PQID | 16002986 |
| PQPubID | 23462 |
| PageCount | 7 |
| ParticipantIDs | proquest_miscellaneous_78896672 proquest_miscellaneous_1627985962 proquest_miscellaneous_16002986 pubmed_primary_9085146 crossref_citationtrail_10_1007_s000110050078 crossref_primary_10_1007_s000110050078 |
| ProviderPackageCode | CITATION AAYXX |
| PublicationCentury | 1900 |
| PublicationDate | 1997-02-01 |
| PublicationDateYYYYMMDD | 1997-02-01 |
| PublicationDate_xml | – month: 02 year: 1997 text: 1997-02-01 day: 01 |
| PublicationDecade | 1990 |
| PublicationPlace | Switzerland |
| PublicationPlace_xml | – name: Switzerland |
| PublicationTitle | Inflammation research |
| PublicationTitleAlternate | Inflamm Res |
| PublicationYear | 1997 |
| SSID | ssj0008282 |
| Score | 1.5711098 |
| Snippet | A comprehensive study to standardise interleukin (IL)-1 alpha, -1 beta, -6, -10, -12 and tumour necrosis factor alpha (TNF alpha) mRNA detection in murine... A comprehensive study to standardise interleukin (IL)-1 alpha , -1 beta , -6, -10, -12 and tumour necrosis factor alpha (TNF alpha ) mRNA detection in murine... Objective and Design: A comprehensive study to standardise interleukin (IL)-1, -1, -6, -10, -12 and tumour necrosis factor alpha (TNF) mRNA detection in murine... |
| SourceID | proquest pubmed crossref |
| SourceType | Aggregation Database Index Database Enrichment Source |
| StartPage | 65 |
| SubjectTerms | Animals Cytokines - biosynthesis Cytokines - genetics Female Interleukin-1 - biosynthesis Interleukin-1 - genetics Interleukin-10 - biosynthesis Interleukin-10 - genetics Interleukin-12 - biosynthesis Interleukin-12 - genetics Interleukin-6 - biosynthesis Interleukin-6 - genetics Lipopolysaccharides - pharmacology Macrophages, Peritoneal - drug effects Macrophages, Peritoneal - metabolism Mice Mice, Inbred BALB C Polymerase Chain Reaction RNA, Messenger - biosynthesis RNA, Messenger - chemistry RNA, Messenger - metabolism Thioglycolates - metabolism Thioglycolates - pharmacology Tumor Necrosis Factor-alpha - biosynthesis Tumor Necrosis Factor-alpha - genetics |
| Title | An investigation of the temporal induction of cytokine mRNAs in LPS-challenged thioglycollate-elicited murine peritoneal macrophages using the reverse transcription polymerase chain reaction |
| URI | https://www.ncbi.nlm.nih.gov/pubmed/9085146 https://www.proquest.com/docview/16002986 https://www.proquest.com/docview/1627985962 https://www.proquest.com/docview/78896672 |
| Volume | 46 |
| hasFullText | 1 |
| inHoldings | 1 |
| isFullTextHit | |
| isPrint | |
| link | http://utb.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwnV1Lj9owELbY3UsvVV-rbh_bqVRxKakWEvI4wgq0rShFu0HiFtnB6aKFBC3hQP9F_1B_W2ds54Fa1McloMRyLM0X-xt75hvG3nHXFo4UiRVw4VhOe-5aXCKR6-BSG_O578uE9iE_j92rqfNp1p01Gt9rUUvbXHyIv_02r-R_rIr30K6UJfsPli07xRv4H-2LV7QwXv_Kxj0KUyx1MjTzIyJp9KZITmOu1WFV9Pguz-6IVK6uxz0VBjua3FhxUU2FAikX2dflTkEjl5ZcLmJFSFe0Iy9J4XhB0t2Ub8Kp8tctJ4GI7abIuCI1qPuNpLITaTUbrbPljna-KC7-lqv0GZ1MUefFH9MEoanTKN8bAaJyo_pmYWJWcBobXJZbRWG2ujO75ZNarHeWrU2giMmomJskP68Igy6nYWQSFvrOF_V52mxVLmrusp50dbEJs3zrgi6_LAw6FmRzoTXyusSMqhWwOPUff4mG09EoCgez8IiddDyPTv5PesN-f1wu7-ii6iN0M0Qj3KryMevd7xOdA96LYjHhI_bQuB_Q01h6zBoyfcKaE61fvmtBWKXjbVrQhEmlbL57yn70UtgDHGQJoOWhAByUgKMnBeBAAQ6fwT7g4ADgQAMOKsBBDXCgAKdeawAHe4CDCnCgAAcF4J6x6XAQXl5ZpgCIFaNfkFt4EZx7Lu9I3pZugGxf2oktE3RLZICeRtvuCNeRgUx4V7STOZ1KuwnyrSARuHTZp-w4xWE-ZxDHjudw8o6d2LmwuRCCUrKR7yMBx07OWKuwVhQbdXwq0rKMSl3vunHPWLNsvtayMIcavilMH-HETadxPJXZdhO11Ym4j29-e7BFxwt8Ko91uBfP9wPX9bDFqcZVOZyAnCnHffHHAbxkD6pv8BU7zu-38jUy7VycsyNv5p2bLwB_-4Px5PonJs3jBQ |
| linkProvider | Library Specific Holdings |
| openUrl | ctx_ver=Z39.88-2004&ctx_enc=info%3Aofi%2Fenc%3AUTF-8&rfr_id=info%3Asid%2Fsummon.serialssolutions.com&rft_val_fmt=info%3Aofi%2Ffmt%3Akev%3Amtx%3Ajournal&rft.genre=article&rft.atitle=An+investigation+of+the+temporal+induction+of+cytokine+mRNAs+in+LPS-challenged+thioglycollate-elicited+murine+peritoneal+macrophages+using+the+reverse+transcription+polymerase+chain+reaction&rft.jtitle=Inflammation+research&rft.au=Simpson%2C+AECM&rft.au=Tomkins%2C+P+T&rft.au=Cooper%2C+K+L&rft.date=1997-02-01&rft.issn=1023-3830&rft.volume=46&rft.issue=2&rft.spage=65&rft.epage=71&rft_id=info:doi/10.1007%2Fs000110050078&rft.externalDBID=NO_FULL_TEXT |
| thumbnail_l | http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/lc.gif&issn=1023-3830&client=summon |
| thumbnail_m | http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/mc.gif&issn=1023-3830&client=summon |
| thumbnail_s | http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/sc.gif&issn=1023-3830&client=summon |