Noninvasive evaluation of liver repopulation by transplanted hepatocytes using31P MRS imaging in mice

Landis, Charles; Yamanouchi, Kaoru; Zhou, Haoran; Mohan, Sankar; Roy‐Chowdhury, Namita; Shafritz, David A.; Koretsky, Alan P.; Roy‐Chowdhury, Jayanta; Hetherington, Hoby P.; Guha, Chandan

doi:10.1002/hep.21382

Cited by 30 publications

(22 citation statements)

References 37 publications

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“…In this case, manganese release from hepatocytes and liver could be exploited as an MR assay of normal liver function. Furthermore, there is also interest in developing MR assays for viability and function of hepatocytes (35) and other cell types (24) incubation of rat liver slices in Mn 2þ , suggest that hepatocytes have three apparently saturable routes for manganese entry. These are (1) a low-affinity mechanism with K ap in the region of 100 mM; (2) a moderately-high-affinity mechanism with K ap in the range of 0.5-2 mM; and (3) a high-affinity mechanism that operates with a K ap of 0.075 mM.…”

Section: Discussionmentioning

confidence: 99%

Manganese cell labeling of murine hepatocytes using manganese(III)‐transferrin

Sotak

Sharer

Koretsky

2008

Contrast Media & Molecular

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Manganese(III)-transferrin [Mn(III)-Tf] was investigated as a way to accomplish manganese-labeling of murine hepatocytes for MRI contrast. It is postulated that Mn(III)-Tf can exploit the same transferrin-receptor-dependent and -independent metabolic pathways used by hepatocytes to transport the iron analog Fe(III)-Tf. More specifically, it was investigated whether manganese delivered by transferrin could give MRI contrast in hepatocytes. Comparison of the T1 and T2 relaxation times of Mn(III)-Tf and Fe(III)-Tf over the same concentration range showed that the r1 relaxivities of the two metalloproteins are the same in vitro, with little contribution from paramagnetic enhancement. The degree of manganese cell labeling following incubation for 2-7 h in 31.5 microm Mn(III)-Tf was comparable to that of hepatocytes incubated in 500 microm Mn2+ for 1 h. The intrinsic manganese tissue relaxivity between Mn(III)-Tf-labeled and Mn2+-labeled cells was found to be the same, consistent with Mn(III) being released from transferrin and reduced to Mn2+. For both treatment regimens, manganese uptake by hepatocytes appeared to saturate in the first 1-2 h of the incubation period and may explain why the efficiency of hepatocyte cell labeling by the two methods appeared to be comparable in spite of the approximately 16-fold difference in effective manganese concentration. Hepatocytes continuously released manganese, as detected by MRI, and this was the same for both Mn2+- and Mn(III)-Tf-labeled cells. Manganese release may be the result of normal hepatocyte function, much in the same way that hepatocytes excrete manganese into the bile in vivo. This approach exploits a biological process-namely receptor binding, endocytosis and endosomal acidification-to initiate the release of an MRI contrast agent, potentially conferring more specificity to the labeling process. The ubiquitous expression of transferrin receptors by eukaryotic cells should make Mn(III)-Tf particularly useful for manganese labeling of a wide variety of cells both in culture and in vivo.

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Section: Discussionmentioning

confidence: 99%

Manganese cell labeling of murine hepatocytes using manganese(III)‐transferrin

Sotak

Sharer

Koretsky

2008

Contrast Media & Molecular

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“…We measured the levels of serum HGF, which is known as a strong stimulator for hepatocytes growth. Although supplying HGF via an adenovirus vector was demonstrated to induce proliferation of transplanted hepatocytes (10,11,14), PVBL did not increase the levels of HGF, as observed in the clinical PVE study (16). Liver regeneration is regulated by an orchestrated and complex response, involving not only HGF, but also various kinds of mediators.…”

mentioning

confidence: 93%

“…Although these results are very attractive, hepatectomy is too invasive to be carried out in patients. Instead of hepatectomy, Fas-mediated apoptosis of host hepatocytes (9) or administration of a recombinant adenovirus vector expressing hepatocyte growth factor (HGF) (10,11) has been successful in inducing massive repopulation of transplanted hepatocytes. However, these strategies appear difficult to implement clinically because of potential toxicity.…”

Section: Introductionmentioning

confidence: 99%

Construction of liver tissue in vivo with preparative partial hepatic irradiation and growth stimulus: investigations of less invasive techniques and progenitor cells

Miyazaki

Yamanouchi

Sakai

et al. 2013

Journal of Surgical Research

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“…Transplants performed in rats have used luciferase imaging to view the engrafted cells; however, this treatment option is not translatable to humans due to the thickness of the abdominal wall. One approach is the use of the creatinine kinase gene as a marker for donor hepatocytes, which when expressed produces phosphocreatinine in the liver and allows for P-31 MRS magnetic resonance imaging of the engrafted donor hepatocytes [84]. Finally, improvements in immunosuppression protocols, or the development of cell-transplantation methods that do not require immunosuppression, would greatly accelerate the field of liver cellular therapy.…”

Section: Cellular Therapiesmentioning

confidence: 99%