RF Field Immunity of a Network Terminating Unit at Over One Gigaherz Frequencies

Työssä tutkitaan telepäätelaitteen yli gigahertsin taajuisen säteilevän RF kentän sietoisuutta. Mittauksissa testattava laite on Tellabs Oy:n valmistaman CTU modeemin tuotekehitysversio. Teoriaosassa käydään läpi sähkömagneettisten aaltojen teoriaa, sekä säteilevän RF kentän aiheuttamien sähkömagneettiset häiriöiden syntymekanismeja. Myös säteilevien häiriöiden EMC mittauksiin tarvittavien mittalaitteiden tärkeimmät ominaisuudet esitellään, sekä pohditaan yli gigahertsin taajuuksille sopivien EMC mittalaitteiden vaatimuksia. EMC standardit eivät tällä hetkellä aseta vaatimuksia telelaitteiden RF kentän sietoisuudelle yli gigahertsin taajuudella. Tämän vuoksi työssä käsitellään myös todennäköisimpiä häiriölähteitä tällä taajuusalueella. Mittauksissa tutkittiin CTU:n RF kentän sietoisuutta taajuusalueella l - 4.2 GHz. Mittaukset suoritettiin sekä radiokaiuttomassa kammiossa että GTEM solussa. Myös metallisten lisäsuojien vaikutusta CTU:n kentänsietoisuuteen tutkittiin GTEM solussa.

Innate and Adaptive Immunity in Orolabial Herpes Simplex

Oral mucosa is a frequent site of primary herpes simplex virus type 1 (HSV-1) infection, whereas intraoral recurrent disease is very rare. Instead, reactivation from latency predominantly results in asymptomatic HSV shedding to saliva or recurrent labial herpes (RLH) with highly individual frequency. The current study aimed to elucidate the role of human oral innate and acquired immune mechanisms in modulation of HSV infection in orolabial region. Saliva was found to neutralize HSV-1, and to protect cells from infection independently of salivary antibodies. Neutralization capacity was higher in saliva from asymptomatic HSV-seropositive individuals compared to subjects with history of RLH or seronegative controls. Neutralization was at least partially associated with salivary lactoferrin content. Further, lactoferrin and peroxidase-generated hypothiocyanite were found to either neutralize HSV-1 or interfere with HSV-1 replication, whereas lysozyme displayed no anti-HSV-1 activity. Lactoferrin was also shown to modulate HSV-1 infection by inhibiting keratinocyte proliferation. RLH susceptibility was further found to be associated with Th2 biased cytokine responses against HSV, and a higher level of anti- HSV-IgG with Th2 polarization, indicating lack of efficiency of humoral response in the control of HSV disease. In a three-dimensional cell culture, keratinocytes were found to support both lytic and nonproductive infection, suggesting HSV persistence in epithelial cells, and further emphasizing the importance of peripheral immune control of HSV. These results suggest that certain innate salivary antimicrobial compounds and Th1 type cellular responses are critically important in protecting the host against HSV disease, implying possible applications in drug, vaccine and gene therapy design.

From Unspecific Quenching to Specific Signaling: Functional GTPase Assays Utilizing Quenching Resonance Energy Transfer (QRET) Technology

The aim of the work presented in this study was to demonstrate the wide applicability of a single-label quenching resonance energy transfer (QRET) assay based on time-resolved lanthanide luminescence. QRET technology is proximity dependent method utilizing weak and unspecific interaction between soluble quencher molecule and lanthanide chelate. The interaction between quencher and chelate is lost when the ligand binds to its target molecule. The properties of QRET technology are especially useful in high throughput screening (HTS) assays. At the beginning of this study, only end-point type QRET technology was available. To enable efficient study of enzymatic reactions, the QRET technology was further developed to enable measurement of reaction kinetics. This was performed using proteindeoxyribonuclei acid (DNA) interaction as a first tool to monitor reaction kinetics. Later, the QRET was used to study nucleotide exchange reaction kinetics and mutation induced effects to the small GTPase activity. Small GTPases act as a molecular switch shifting between active GTP bound and inactive GDP bound conformation. The possibility of monitoring reaction kinetics using the QRET technology was evaluated using two homogeneous assays: a direct growth factor detection assay and a nucleotide exchange monitoring assay with small GTPases. To complete the list, a heterogeneous assay for monitoring GTP hydrolysis using small GTPases, was developed. All these small GTPase assays could be performed using nanomolar protein concentrations without GTPase pretreatment. The results from these studies demonstrated that QRET technology can be used to monitor reaction kinetics and further enable the possibility to use the same method for screening.