Exercise training increases K+-channel contribution to regulation of coronary arterial tone

The present study examined whether regulation ofcoronary tone in conduit arteries (>1.0 mm ID) is altered by exercisetraining. Yucatan miniature swine were treadmill trained for 16-20wk (Ex) and compared with sedentary counterparts (Sed).Endothelium-denuded arterial rings were stretched to optimal length andallowed to equilibrate for 60 min. Inhibition of eitherCa²⁺-activated channels [1mM tetraethylammonium (TEA) or 10 nM iberiotoxin (IBTX)] orvoltage-dependent K⁺ channels[1 mM 4-aminopyridine (4-AP)] significantlyincreased resting tension in both groups; however, the effect of allK⁺-channel blockers was greater inEx. Addition of 1 mM sodium nitroprusside reduced resting tension inboth groups, confirming the presence of active basal tone; however,sodium nitroprusside-sensitive tone was increased approximately twofoldin Ex compared with Sed group. Perforated patch-clamp experiments onisolated smooth muscle cells demonstrated no effect of exercisetraining on whole cell TEA-sensitive, 4-AP-sensitive, or basalK⁺ current. Similarly, whereasTEA, 4-AP, and IBTX all decreased resting membrane potential, there wasno difference in depolarization between groups. The greater effect ofTEA on resting tension in Ex could be mimicked in Sed by addition ofthe Ca²⁺-channel agonist BAY K8644. In conclusion, the greater response toK⁺-channel blockers after exercisetraining is consistent with an increased contribution ofK⁺ channels to regulation of basaltone in conduit coronary arteries. The lack of an effect of training onK⁺ current characteristics ormembrane potential responses in isolated cells suggests that arequisite factor for enhancedK⁺-channel activation in arteriesfrom Ex, possibly stretch, is absent in isolated cells.

     

Generation and characterization of a Ddx4-iCre transgenic line for deletion in the germline beginning at genital ridge colonization

Germline-specific Cre lines are useful for analyses of primordial germ cell, spermatogonial and oogonial development, but also for whole-body deletions when transmitted through subsequent generations. Several germ cell specific Cre mouse strains exist, with various degrees of specificity, efficiency, and temporal activation. Here, we describe the CRISPR/Cas9 targeted insertion of an improved Cre (iCre) sequence in-frame at the 3′ end of the Ddx4 locus to generate the Ddx4-P2A-iCre allele. Our functional assessment of this new allele, designated Ddx4^iCreJoBo, reveals that Cre activity begins in PGCs from at least E10.5, and that it achieves higher efficiency for early gonadal (E10.5–12.5) germline deletion when compared to the inducible Oct4^CreERT2 line. We found the Ddx4^iCreJoBo allele to be hypomorphic for Ddx4 expression and homozygous males, but not females, were infertile. Using two reporter lines (R26R^LacZ and R26R^tdTomato) and a floxed gene of interest (Cripto^flox) we found ectopic activity in multiple organs; global recombination (a common feature of germline Cre alleles) varies from 10 to 100%, depending on the particular floxed allele. There is a strong maternal effect, and therefore it is preferable for Ddx4^iCreJoBo to be inherited from the male parent if ubiquitous deletion is not desired. With these limitations considered, we describe the Ddx4^iCreJoBo line as useful for germline studies in which early gonadal deletion is required.     

Endopeptidase activity in jackbeans and its effect on Concanavalin A

Endopeptidase activity in mature jackbeans has been characterised. One major activity is present, that of a neutral metallo-endopeptidase. Using specific inhibitors it can be shown that the Concanavalin A-associated fragments are not formed by proteolytic degradation of the intact subunit on hydration of the tissue. The intact subunit of the lectin is also resistant to the degradation by the endogenous endopeptidase activity during a prolonged incubation in vitro. These results suggest that the lectin fragments have been formed during seed maturation and no further limited proteolysis of Concanavalin A occurs during the early stages of germination.     

Liposomal-delivery of phosphodiesterase 5 inhibitors augments UT-15C-stimulated ATP release from human erythrocytes

The use of liposomes to affect targeted delivery of pharmaceutical agents to specific sites may result in the reduction of side effects and an increase in drug efficacy. Since liposomes are delivered intravascularly, erythrocytes, which constitute almost half of the volume of blood, are ideal targets for liposomal drug delivery.In vivo, erythrocytes serve not only in the role of oxygen transport but also as participants in the regulation of vascular diameter through the regulated release of the potent vasodilator, adenosine triphosphate (ATP). Unfortunately, erythrocytes of humans with pulmonary arterial hypertension (PAH) do not release ATP in response to the physiological stimulus of exposure to increases in mechanical deformation as would occur when these cells traverse the pulmonary circulation. This defect in erythrocyte physiology has been suggested to contribute to pulmonary hypertension in these individuals.In contrast to deformation, both healthy human and PAH erythrocytes do release ATP in response to incubation with prostacyclin analogs via a well-characterized signaling pathway. Importantly, inhibitors of phosphodiesterase 5 (PDE5) have been shown to significantly increase prostacyclin analog-induced ATP release from human erythrocytes.Here we investigate the hypothesis that targeted delivery of PDE5 inhibitors to human erythrocytes, using a liposomal delivery system, potentiates prostacyclin analog- induced ATP release. The findings are consistent with the hypothesis that directed delivery of this class of drugs to erythrocytes could be a new and important method to augment prostacyclin analog-induced ATP release from these cells. Such an approach could significantly limit side effects of both classes of drugs without compromising their therapeutic effectiveness in diseases such as PAH.