Your search keyword '"Milner, Anne E."' showing total 4 results

1. Three restricted forms of Epstein--Barr virus latency counteracting apoptosis in c-myc-expressing Burkitt lymphoma cells.

Author

Kelly, Gemma L., Milner, Anne E., Baldwin, Gouri S., Bell, Andrew I., and Rickinson, Alan B.

Subjects

*EPSTEIN-Barr virus, *B cells, *MEMBRANE proteins, *BURKITT'S lymphoma, *APOPTOSIS, *ANTIGENS

Abstract

Epstein-Barr virus (EBV), a human herpesvirus, transforms B cell growth in vitro through expressing six virus-coded Epstein-Barr nuclear antigens (EBNA5) and two latent membrane proteins (LMPs). In many EBV-associated tumors, however, viral antigen expression is more restricted, and the aetiological role of the virus is unclear. For example, endemic Burkitt lymphoma (BL) classically presents as a monoclonal, c-myc-translocation-positive tumor in which every cell carries EBV as an EBNA1-only (Latency I) infection; such homogeneity among EBV-positive cells, and the lack of EBV-negative comparators, hampers attempts to understand EBV's role in BL pathogenesis. Here, we describe an endemic BL that was unusually heterogeneous at the single-cell level and, in early passage culture, yielded a range of cellular clones, all with the same c-myc translocation but differing in EBV status. Rare EBV-negative cells were isolated alongside EBV-positive cells displaying one of three forms of restricted latency: (,) conventional Latency I expressing EBNA1 only from a WI virus genome, (ii) Wp-restricted latency expressing EBNAs 1, 3A, 3B, 3C, and-IP only from an EBNA2-deleted genome, and (iii) a previously undescribed EBNA2+/LMP1- latency in which all six EBNA5 are expressed again in the absence of the LMP5. Intercional comparisons showed that each form of EBV infection was associated with a specific degree of protection from apoptosis. Our work suggests that EBV acts as an antiapoptotic rather than a growth-promoting agent in BL by selecting among three transcriptional programs, all of which, unlike the full virus growth-transforming program, remain compatible with high c-myc expression. [ABSTRACT FROM AUTHOR]

Published

2006

2. Differential effects of BCL-2 on survival and proliferation of human B-lymphoma cells following γ-irradiation.

Author

Milner, Anne E, Grand, Roger JA, Vaughan, Andrew TM, Armitage, Richard J, and Gregory, Christopher D

Subjects

*B cell lymphoma, *LYMPHOMAS, *CANCER cells, *CELL proliferation, *APOPTOSIS

Abstract

Bcl-2 can inhibit apoptosis induced by a variety of stimuli, including radiation and its presence in tumour cells would be expected to indicate poor prognosis. Bcl-2-expressing tumours, however, are often low-grade and highly responsive to therapy. To investigate this apparent paradox, we analysed in vitro the responses of Burkitt lymphoma (BL) cells to γ-irradiation in the presence and absence of Bcl-2. High-level expression of Bcl-2 was shown to promote BL cell survival following irradiation. However, a significant proportion of Bcl-2-rescued cells subsequently underwent apoptosis after an extended period in culture. In addition, in different BL lines, Bcl-2 was found either to promote or to inhibit long-term proliferative activity following γ-irradiation. This differential regulation of proliferation correlated both with differential effects of Bcl-2 on the cell cycle and with differences in p53 status. Thus, by one week after irradiation, BL cells expressing only wild-type p53 (wt/wt) had arrested in G1, whereas those with a mutant allele (wt/mu) were arrested in all phases of the cell cycle. The proportion of Bcl-2-rescued cells that subsequently underwent apoptosis was reduced by ligation of CD40 at the time of irradiation in wt/wt BL cells, but not in wt/mu cells. CD40-ligation reduced both G1-arrest and apoptosis in parallel. These results indicate that, whilst Bcl-2 can delay apoptosis in BL cells following γ-irradiation, the protein can also cause growth-arrest and thereby promote apoptosis. Long-term survival following Bcl-2-mediated rescue of γ-irradiated cells may depend on p53 status and require additional death-repressing or growth-promoting signals. [ABSTRACT FROM AUTHOR]

Published

1997

3. Adenovirus early region 1A protein binds to mammalian SUG1-a regulatory component of the proteasome.

Author

Grand, Roger JA, Turnell, Andrew S, Mason, Grant GF, Wang, Wenlan, Milner, Anne E, Mymryk, Joe S, Rookes, Susan M, Rivett, A Jennifer, and Gallimore, Phillip H

Subjects

*ADENOVIRUS diseases, *PROTEOLYTIC enzymes, *CARCINOGENESIS, *PROTEINS

Abstract

Adenovirus early region 1A (Ad E1A) is a multifunctional protein which is essential for adenovirus-mediated transformation and oncogenesis. Whilst E1A is generally considered to exert its influence on recipient cells through regulation of transcription it also increases the level of cellular p53 by increasing the protein half-life. With this in view, we have investigated the relationship of Ad E1A to the proteasome, which is normally responsible for degradation of p53. Here we have shown that both Ad5 and Ad12 E1A 12S and 13S proteins can be co-immunoprecipitated with proteasomes and that the larger Ad12 E1A protein binds strongly to at least three components of the 26S but not 20S proteasome. One of these interacting species has been identified as mammalian SUG1, a proteasome regulatory component which also plays a role in the cell as a mediator of transcription. In vitro assays have demonstrated a direct interaction between Ad12 E1A 13S protein and mouse SUG1. Following infection of human cells with Ad5 wt and Ad5 mutants with lesions in the E1A gene it has been shown that human SUG1 can be co-immunoprecipitated with full-length E1A and with E1A carrying a deletion in conserved region 1 which is the region considered to be responsible for increased expression of p53. We have concluded therefore that Ad E1A binds strongly to SUG1 but that this interaction is not responsible for inhibition of proteasome activity. This is consistent with the observation that purified Ad12 E1A inhibits the activity of the purified 20S but not 26S proteasomes. We have also demonstrated that SUG1 can be co-immunoprecipitated with SV40 T and therefore we suggest that this may represent a common interaction of transforming proteins of DNA tumour viruses. [ABSTRACT FROM AUTHOR]

Published

1999

4. Control of human B-lymphocyte replication. I. CHARACTERIZATION OF NOVEL ACTIVATION STATES THAT PRECEDE THE ENTRY OF Go B CELLS INTO CYCLE.

Author

Walker, Leonie, Guy, G., Brown, G., Rowe, M., Milner, Anne E., and Gordon, J.

Subjects

*IMMUNOGLOBULINS, *LYMPHOCYTES, *B cells, *GENES, *PHOSPHOLIPIDS, *STAPHYLOCOCCUS aureus

Abstract

Tonsillar B lymphocytes of a particularly high buoyant density were prepared essentially free of contaminating monocytes and T cells. When exposed to anti-immunoglobulin, such cells initiated the hydrolysis of inositol phospholipids. This provides a postulated `dual signal' for growth through the liberation of intracellular calcium stores and the activation of protein kinase C. Nevertheless, neither anti-immunoglobulin nor direct agonists of this bifurcating pathway (respectively, calcium ionophore and the phorbol ester TPA) were capable, when used alone, of driving cells out of G0 and into RNA synthesis. All three agents did, however, induce two activation antigens at the surface of G0 B cells, which included CD23, p45 and a lineage-unrestricted antigen identified by the monoclonal antibody BK. 19.9. Cells that had been exposed to calcium ionophore, but not those activated with either TPA or anti-immunoglobulin, revealed further change indicated by an increased accessibility of their native DNA for the intercalating dye acridine orange. Cells receiving full mitogenic signals in the form of Staphylococcus aureus Cowan Strain I (SAC) or a combination of TPA and calcium ionophore showed the same initial sequelae but continued to enter the cell cycle and progress through to DNA synthesis. The observations identify two phases in the early activation of human B cells, both in terms of various temporal events, and the signals required to promote each activation state. Furthermore, cells receiving complete growth signals were required to transit these activation states before entering the proliferative cycle. Thus, the exit of human B cells from G0, appears subject to multiple controls that precede those associated with G1 and later phases of the cell cycle. [ABSTRACT FROM AUTHOR]

Published

1986