ABSTRACT
Novel 2D material-based supercapacitors are promising candidates for energy applications due to their distinctive physical, chemical, and electrochemical properties. In this study, a dandelion-like structure material comprised of Sm2O3, Co3O4, and 2D reduced graphene oxide (rGO) on nickel foam (NF) was synthesised using a hydrothermal method followed by subsequent annealing treatment. This dandelion composite grows further through the tremella-like structure of Sm2O3 and Co3O4, which facilitates the diffusion of ions and prevents structural collapse during charging and discharging. A substantial number of active sites are generated during redox reactions by the unique surface morphology of the Sm2O3/Co3O4/rGO/NF composite (SCGN). The maximum specific capacity the SCGN material achieves is 3448 F g-1 for 1 A g-1 in a 6 mol L-1 KOH solution. Benefiting from its morphological structure, the prepared composite (SCGN) exhibits a high cyclability of 93.2% over 3000 charge-discharge cycles at 10 A g-1 and a coulombic efficiency of 97.4%. Additionally, the assembled SCGN//SCGN symmetric supercapacitors deliver a high energy density of 64 W h kg-1 with a power density of 300 W kg-1, which increases to an outstanding power density of 12 000 W kg-1 at 28.7 W h kg-1 and long cycle stability (80.9% capacitance retention after 30 000 cycles). These results suggest that the manufactured SCGN electrodes could be viable active electrode materials for electrochemical supercapacitors.
ABSTRACT
PURPOSE: Tubo-ovarian cancer (TOC) is a sentinel cancer for BRCA1 and BRCA2 pathogenic variants (PVs). Identification of a PV in the first member of a family at increased genetic risk (the proband) provides opportunities for cancer prevention in other at-risk family members. Although Australian testing rates are now high, PVs in patients with TOC whose diagnosis predated revised testing guidelines might have been missed. We assessed the feasibility of detecting PVs in this population to enable genetic risk reduction in relatives. PATIENTS AND METHODS: In this pilot study, deceased probands were ascertained from research cohort studies, identification by a relative, and gynecologic oncology clinics. DNA was extracted from archival tissue or stored blood for panel sequencing of 10 risk-associated genes. Testing of deceased probands ascertained through clinic records was performed with a consent waiver. RESULTS: We identified 85 PVs in 84 of 787 (11%) probands. Familial contacts of 39 of 60 (65%) deceased probands with an identified recipient (60 of 84; 71%) have received a written notification of results, with follow-up verbal contact made in 85% (33 of 39). A minority of families (n = 4) were already aware of the PV. For many (29 of 33; 88%), the genetic result provided new information and referral to a genetic service was accepted in most cases (66%; 19 of 29). Those who declined referral (4 of 29) were all male next of kin whose family member had died more than 10 years before. CONCLUSION: We overcame ethical and logistic challenges to demonstrate that retrospective genetic testing to identify PVs in previously untested deceased probands with TOC is feasible. Understanding reasons for a family member's decision to accept or decline a referral will be important for guiding future TRACEBACK projects.
Subject(s)
Breast Neoplasms , Ovarian Neoplasms , Australia , Breast Neoplasms/genetics , Carcinoma, Ovarian Epithelial/genetics , Family , Female , Genetic Predisposition to Disease , Genetic Testing/methods , Humans , Male , Ovarian Neoplasms/genetics , Ovarian Neoplasms/prevention & control , Pilot Projects , Retrospective StudiesABSTRACT
Anal cancer is a rare disease that has doubled in incidence over the last four decades. Current treatment and survival of patients with this disease has not changed substantially over this period of time, due, in part, to a paucity of preclinical models to assess new therapeutic options. To address this hiatus, we set-out to establish, validate and characterise a panel of human anal squamous cell carcinoma (ASCC) cell lines by employing an explant technique using fresh human ASCC tumour tissue. The panel of five human ASCC cell lines were validated to confirm their origin, squamous features and tumourigenicity, followed by molecular and genomic (whole-exome sequencing) characterisation. This panel recapitulates the genetic and molecular characteristics previously described in ASCC including phosphoinositide-3-kinase (PI3K) mutations in three of the human papillomavirus (HPV) positive lines and TP53 mutations in the HPV negative line. The cell lines demonstrate the ability to form tumouroids and retain their tumourigenic potential upon xenotransplantation, with varied inducible expression of major histocompatibility complex class I (MHC class I) and Programmed cell death ligand 1 (PD-L1). We observed differential responses to standard chemotherapy, radiotherapy and a PI3K specific molecular targeted agent in vitro, which correlated with the clinical response of the patient tumours from which they were derived. We anticipate this novel panel of human ASCC cell lines will form a valuable resource for future studies into the biology and therapeutics of this rare disease.
