Universality and robustness of revivals in the transverse field XY model

We study the structure of the revivals in an integrable quantum many-body system, the transverse field XY spin chain, after a quantum quench. The time evolutions of the Loschmidt echo, the magnetization, and the single-spin entanglement entropy are calculated. We find that the revival times for all of these observables are given by integer multiples of T-rev similar or equal to L/upsilon(max), where L is the linear size of the system and upsilon(max) is the maximal group velocity of quasiparticles. This revival structure is universal in the sense that it does not depend on the initial state and the size of the quench. Applying nonintegrable perturbations to the XY model, we observe that the revivals are robust against such perturbations: they are still visible at time scales much larger than the quasiparticle lifetime. We therefore propose a generic connection between the revival structure and the locality of the dynamics, where the quasiparticle speed upsilon(max) generalizes into the Lieb-Robinson speed upsilon(LR)

Progesterone-induced blocking factor differentially regulates trophoblast and tumor invasion by altering matrix metalloproteinase activity

Invasiveness is a common feature of trophoblast and tumors; however, while tumor invasion is uncontrolled, trophoblast invasion is strictly regulated. Both trophoblast and tumor cells express high levels of the immunomodulatory progesterone-induced blocking factor (PIBF), therefore, we aimed to test the possibility that PIBF might be involved in invasion. To this aim, we used PIBF-silenced or PIBF-treated trophoblast (HTR8/Svneo, and primary trophoblast) and tumor (HT-1080, A549, HCT116, PC3) cell lines. Silencing of PIBF increased invasiveness as well as MMP-2,-9 secretion of HTR8/SVneo, and decreased those of HT-1080 cells. PIBF induced immediate STAT6 activation in both cell lines. Silencing of IL-4Rα abrogated all the above effects of PIBF, suggesting that invasion-related signaling by PIBF is initiated through the IL-4Rα/PIBF-receptor complex. In HTR-8/SVneo, PIBF induced fast, but transient Akt and ERK phosphorylation, whereas in tumor cells, PIBF triggered sustained Akt, ERK, and late STAT3 activation. The late signaling events might be due to indirect action of PIBF. PIBF induced the expression of EGF and HB-EGF in HT-1080 cells. The STAT3-activating effect of PIBF was reduced in HB-EGF-deficient HT-1080 cells, suggesting that PIBF-induced HB-EGF contributes to late STAT3 activation. PIBF binds to the promoters of IL-6, EGF, and HB-EGF; however, the protein profile of the protein/DNA complex is different in the two cell lines. We conclude that in tumor cells, PIBF induces proteins, which activate invasion signaling, while—based on our previous data—PIBF might control trophoblast invasion by suppressing proinvasive genes.Hungarian National Research Fund (OTKA 77717), from theUniversity of Pecs (34039/KA-PostDoc12-03) and by TÁMOP-4.2.1/B-10/1-2010-0002.Deposited by bulk impor