LAM cells biology and lymphangioleiomyomatosis.

[lymphangioleiomyomatosis]

Progressive lung tissue destruction in lymphangioleiomyomatosis (LAM ) occurs as a result of excessive proliferation of LAM cells caused by a mutation in one of the tuberous sclerosis complex suppressor genes , TSC 1 or TSC 2 . These cells show constitutive activation of the mammalian target of rapamycin (mTOR ) pathway and many of the mTOR-related kinases such as Akt , Erk , S 6 K 1 and S 6 . Phenotype of LAM cells differs considerably depending on their microenvironment . LAM cells show differences in morphology , size and expression of various factors depending on their location in the tumor or body fluids . The presence of LAM cells in blood , urine , bronchoalveolar lavage fluid (BALF ), and chyle proves their ability to metastasis . Antigens of smooth muscle cells are expressed in most LAM cells . Some of these cells are immunoreactive with HMB-45 antibody , which is used for the immunohistochemical diagnosis of LAM . Receptors for estrogen and progesterone may also be expressed in these cells , which probably is associated with the fact that LAM occurs almost exclusively in women of childbearing age . LAM cells via increased production of metalloproteinases are involved in the destruction of the extracellular matrix , as well as the remodeling and damage of lung tissue . Sporadic LAM occurs extremely rarely . Therefore a good experimental model of this disease is necessary . To date , several animal and human cell lines , which both genetically and phenotypically resemble LAM cells , have been obtained . These cell lines , derived from LAM nodule or an angiomyolipoma , are usually characterized by a mutation of the TSC 2 gene , expression of smooth muscle cell antigens such as a-smooth muscle actin (aSMA ) or S 6 K 1 and S 6 protein hyperphosphorylation . Presently , there is no commercially available cell line representing a good model of LAM . A better understanding of LAM cell biology is necessary for creating a useful model in vitro for further exploration of both LAM pathomechanisms and more general mechanisms of carcinogenesis .