Maintenance of insulin release from pancreatic islets stored in the cold for up to 5 weeks.

Frankel, Barbara J.; Gylfe, Erik; Hellman, Bo; Idahl, L

doi:10.1172/jci108267

Cited by 42 publications

(19 citation statements)

References 15 publications

(15 reference statements)

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“…This phenomenon has been observed previously by Frankel et al, 8 who used a static culture system, and Rabinovitch et al, 9 who used static cultures subsequently transferred to a perifusion system for study. The cause for this decrease in secretory rate of insulin from cultured islets is unknown.…”

Section: Discussionsupporting

confidence: 74%

Insulin and Glucagon Secretion from Rat Islets Maintained in a Tissue Culture-Perifusion System

et al. 1979

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A tissue culture-perifusion system is described that allows for long-term culture of pancreatic islets and study of the dynamics of islet hormone secretion. Islets cultured in this system demonstrate brisk, reproducible biphasic insulin and glucagon release. Glucose-stimulated insulin release is similar after 1 or 14 days in culture. Freshly isolated islets are relatively insensitive to somatostatin, requiring 100 ng/ml to suppress partially the glucose-induced insulin secretion. After 24 h of culture, the same islets demonstrate a marked increase in sensitivity to this hormone. Glucagon secretion from islets maintained in this system occurred in a predictable fashion to arginine stimulation and glucose inhibition.

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Section: Discussionsupporting

confidence: 74%

Insulin and Glucagon Secretion from Rat Islets Maintained in a Tissue Culture-Perifusion System

et al. 1979

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“…Measurement of cAMP levels in the cultures revealed dissociations between effects on B cell replication and insulin release. Thus, addition of 0.1 mM IBMX, or 0.1 nM cholera toxin, to 5.6 mM glucose produced slightly greater increases in cAMP levels and B cell replication than did 16.7 mM glucose, whereas insulin release was increased significantly more with 16 (15-20 mM) has been shown to increase glucose metabolism (1, 2), insulin release and content (3)(4)(5)(6), and insulin biosynthesis (7), and also to improve the survival (6) and to stimulate the replication (8)(9)(10)(11) of islet B cells. Glucose has also been reported to stimulate adenylate cyclase (5,12) and to increase cyclic adenosine-3',5'-monophosphate (cAMP) levels (13) Green ancd Taylor (26).…”

mentioning

confidence: 93%

Cyclic Adenosine-3′,5′ -monophosphate Stimulates Islet B Cell Replication in Neonatal Rat Pancreatic Monolayer Cultures

Rabinovitch¹,

Blondel²,

Murray³

et al. 1980

J. Clin. Invest.

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“…The yield obtained with present methods for islet isolation is therefore insuffi cient for healing diabetes by transplantation. Previous investigations have suggested two possible ways to circumvent the problem of the low yield; the use of several donors and long-term storage [7,9,20,24] or repeated transplantation [18]. The separation of pancreatic islets from collagenasedigested pancreas by sedimentation through Percoll at unit gravity might also obviate the problem of the low yield; this method by its simplicity being suitable for large-scale islet isolation [5].…”

Section: Discussionmentioning

confidence: 99%

“…18-24 h elapsed between islet isola tion and the efflux experiments. Since during this time the islets were stored at room temperature or in a refrigerator, they were allowed to recover at 37 °C for 2-4 h [9] before the experiments.…”

Section: Methodsmentioning

confidence: 99%

Collagenase Isolation and <sup>45</sup>Ca Efflux Studies of Human Islets of Langerhans

Henriksson¹,

G²,

Gylfe³

et al. 1978

Eur Surg Res

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22 human pancreases were removed soon after circulatory arrest from donors aged 15–63 years. Part of the pancreas was used for isolation of islets by the collagenase technique. The mean yield + SEM, expressed as the number of islets isolated from 4 g pancreas was 79 + 15. The yield varied considerably even when the pancreas was removed immediately after circulatory arrest and the histology was normal, and there was no correlation with the age of the donors. The islet content of insulin (ng/µg dry islet) was 8.5 + 1.2 (mean + SEM). Isolated islets were loaded with ^4sCa in the presence of 20 mM glucose and placed in a perfusion apparatus for further studies of the ⁴⁵Ca washout. The decrease of washout of radioactivity in Ca²⁺-deficient medium offers support for the existence of a Ca²⁺-Ca²⁺ exchange process. When added in a concentration of 20 mM, glucose tended to stimulate ⁴⁵Ca efflux in perfusion medium of ordinary ionic composition but inhibited this process when the medium was deficient in Ca²⁺. Exposure to the calcium ionophore X-537A resulted in immediate stimulation of ⁴⁵Ca efflux from human islets as previously observed for islets from rats and mice. This suggests that Ca²⁺ has a direct regulatory role for insulin release also in humans.

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Maintenance of insulin release from pancreatic islets stored in the cold for up to 5 weeks.

Cited by 42 publications

References 15 publications

Insulin and Glucagon Secretion from Rat Islets Maintained in a Tissue Culture-Perifusion System

Insulin and Glucagon Secretion from Rat Islets Maintained in a Tissue Culture-Perifusion System

Cyclic Adenosine-3′,5′ -monophosphate Stimulates Islet B Cell Replication in Neonatal Rat Pancreatic Monolayer Cultures

Collagenase Isolation and <sup>45</sup>Ca Efflux Studies of Human Islets of Langerhans

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