Assessment of Ascorbic Acid Effects on the Properties of Cell-Derived Tissue Rings

Hu, Jason Z

24 June 2010

"We have developed a system to rapidly create three-dimensional tissue rings from aggregated cells. The ability to use cell-derived tissues to screen the effects of culture conditions on tissue mechanical function has not previously been reported. The first goal of this study was to evaluate the mechanical properties of cell-derived tissue rings in response to ascorbic acid, which has been shown to increase collagen content, resulting in increased mechanical strength. The second goal was to develop quantitative methods to evaluate the structure and composition of cell-derived tissue rings. Rat aortic smooth muscle cells (1.33x10^6 cells/ring) were seeded in agarose wells with 4 mm post diameters in DMEM supplemented with 10% FBS and ascorbic acid (0, 50, 150 ug/ml). After 7 days, the average thickness of the constructs reached 0.72 +/- 0.03 mm with no statistical differences between groups. Ultimate tensile strength values were higher in the ascorbic acid-treated groups compared to untreated controls. However, there was no significant difference between tissue rings treated with 50 and 150 ug/ml ascorbic acid. Biochemical analysis showed that ascorbic acid did not significantly affect total protein, collagen content or cell number. Image analysis of polarized light micrographs suggested that collagen fibril coverage increased in response to ascorbic acid treatment, although the differences between groups were insignificant. In addition to ascorbic acid treatment, we also subjected tissue rings to DTPA treatment to prolong ascorbic acid availability in culture medium, which resulted in weak and necrotic tissue rings. Reduced serum was also investigated in order to decrease cell proliferation, which resulted in decreased tissue thickness and increased mechanical strength. Overall, we successfully demonstrated that the mechanical properties of the tissue rings could be altered by ascorbic acid treatment, and developed a series of quantitative methods to measure tissue mechanics, composition and organization. The results of this study further support the potential to use the tissue ring system as a high throughput screening method for studying the functional properties of three-dimensional engineered tissues."

CDM

ascorbic acid

tissue engineering

collagen

RASMCs

TEBVs

JAK/STAT signalling in the induction of the L-arginine-nitric oxide pathway in macrophages and vascular smooth muscle cells

Garr, Edmund Dzigbordi

January 2014

The production of Nitric Oxide (NO) under physiological conditions has beneficial roles in acting as a key signaling component of many biological processes as well as having an anti-microbial effect. However its effects following excess production by the inducible NO pathway is potentially detrimental in the pathogenesis of chronic inflammation including sepsis and several other inflammatory diseases. Understanding the mechanisms that regulate the expression of the inducible nitric oxide synthase (iNOS) responsible for producing the excessive amounts of NO in disease states is therefore critical. In this regards, experiments were carried out to identify the signaling pathways that may mediate this process, focusing specifically on the JAK/STAT cascade. The reason for selecting the latter is because our research group, amongst others, has carried out extensive work investigating other signaling pathways, including the mitogen activated kinases (MAPK). Moreover, studies have also been carried out in an attempt to identify the critical role of JAK/STAT signaling for iNOS induction. These studies however failed to conclusively demonstrate whether, as with the MAPKs, the JAK/STATs may also play an essential role. Furthermore there is indeed controversy in the literature with researchers unable to agree whether expression of iNOS does require JAK/STAT activation. Thus, the aim of the project described in this thesis was to establish unequivocally whether activation of the JAK/STATs preceeds induction of iNOS. The studies were extended to L-arginine transport as well because the latter is widely reported to be induced in parallel with iNOS and substrate supply to iNOS may be critical for sustained NO production. Changes in transporter activity as well as their expression profiles were assessed. All experiments were carried out in either rat aortic smooth muscle cells (RASMCs) or in the J774 macrophage cell line. These cell types were selected because RASMCs are one of the prime targets for induced NO production in vascular inflammation and the macrophages are involved in host defence, acting in part through NO production. To establish the role of JAK/STATs, pharmacological and molecular approaches were used. Pharmacologically, two inhibitors were used and these were AG490 and JAK inhibitor I. The former is reported to be a selective JAK2 inhibitor and the other blocks all known JAK proteins. The potential of the GTPases to regulate the induction of iNOS was also examined using selective inhibitor known to regulate these proteins. In addition to these drugs, siRNA targeting JAK2 was also exploited and western blotting was extensively used to detect expression of various proteins including iNOS, native and phosphorylated JAK2 and TYK2. Changes in iNOS activity was monitored by determining nitrite production using the Griess assay and L-arginine transport was monitored using tritiated arginine (L-[3H]arginine). RASMCs were treated with a combination of LPS (100 µg/ml) and IFN- (100 U/ml) and the macrophages with LPS (1 µg/ml) to induce iNOS and transporter activity. Consistent with previous reports, the above treatment of both cell types resulted in the expression of iNOS, production of NO and enhanced transport of L-arginine. These effects were not affected by AG490 but blocked by JAK inhibitor I. Furthermore, although both cell types expressed the key JAKs (JAK2 and TYK2), neither of these proteins were phosphorylated under conditions of induced NO production. Moreover, siRNA experiments showed that JAK2 expression could be abolished without any significant change in NO production, confirming that at least JAK2 may not be required for this process. Whether TYK2 is involved still remains to be resolved as the phosphor-protein could not be detected. However the conclusive siRNA knockdown studies could not be carried out due to time and cost constraints. Apart from iNOS and NO production, changes in induced L-arginine transport were also not significantly affected under the experimental conditions described above suggesting that like with iNOS, induction of L-arginine transport is independent of at least JAK2. Interestingly however, STAT-1 was phosphorylated and this was blocked by JAK inhibitor I but not AG490. Thus, STAT-1 activation may be essential but its activation may be independent of the JAKs. One possible alternate upstream activator of STAT-1 may be the GTPases. Indeed these proteins have been indicated to phosphorylate STAT-1 independent of the JAKs. However, in this project, inhibition of the GTPase pathway enhanced NO production and L-arginine transport suggesting that the GTPases downregulate these processes. In conclusion, the studies carried out in this thesis have shown that induction of iNOS, NO production and L-arginine transport in both RASMCs and J774 macrophages are independent of JAK2 but require STAT-1 activation which may be phosphorylated independently of the JAKs. The role of other JAKs such as TYK2 although unlikely, will need to be resolved using a more specific approach such as siRNA.

616.07