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Objective:To observe the lipogenic or osteogenic differentiation of decellularized adipose matrix (DAM) in the periosteal microenvironment.Methods:From June 2020 to December 2020, adipose tissue obtained by human liposuction was prepared as DAM at the National Institute of Plastic Surgery. Six male SD rats of 4 to 6 weeks were selected and implanted into the subperiosteum of the rat parietal bone according to the same initial volume. After 12 weeks, adipogenesis and osteogenic differentiation of DAM were observed by gross specimens, histological staining, and immunofluorescence staining. Label-free quantitative protein mass spectrometry was used for detection of osteogenic-associated proteins in DAM.Results:Vascularization around the DAM was evident. Adipogenesis and angiogenesis were observed in DAM by H&E and Masson staining, while OCN immunofluorescence staining confirmed osteogenic differentiation of DAM. The osteogenic differentiation related proteins were screened by mass spectrometry.Conclusions:In the microenvironment of periosteum, DAM mainly differentiates towards adipose tissue, but a few of them havs the potential to differentiate towards osteogenesis, which might be related to some of the osteogenesis-related proteins contained in DAM.
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Resumen La espectrometría de masas MALDI-TOF MS es una técnica rápida y sencilla para identificar microorganismos por análisis proteico. Se estudiaron 304 aislados de levaduras procedentes de micosis superficiales y profundas, con el objetivo de comparar tres métodos: convencional (bioquímico y morfológico), MALDI-TOF MS, y reacción en cadena de la polimerasa (RPC, método de referencia). Se estudiaron 24 especies con predominio de Candida spp y Cryptococcus spp. La identificación por método convencional fue de 258/304 cepas, mientras que por MALDI-TOF MS fue de: 277/304 cepas (84,8 versus 91,2%, p = no significativo). El coeficiente Kappa entre el MALDI-TOF MS y la RPC reportó una excelente concordancia (0,99). La sensibilidad y la especificidad de MALDI-TOF MS para la identificación de levaduras patógenas oportunistas de muestras clínicas fueron de 94,6% y 99%; respectivamente. MALDI-TOF MS demostró ser una herramienta de alta precisión para la identificación de levaduras patógenas.
MALDI-TOF MS mass spectrometry is a rapid and straightforward technique to identify microorganisms by protein analysis. The study was performed in 304 yeast isolates from superficial and deep mycoses, in order to compare three methods: conventional (biochemical and morphological), MALDI-TOF MS, and polymerase chain reaction (PCR, reference). We included 24 species with predominance of Candida spp and Cryptococcus spp. The identification by conventional methods was 258/304 strains, while by MALDI-TOF MS was: 277/304 strains (84.8% versus 91.2%, P = not significant). The Kappa coefficient comparing MALDI-TOF-MS with PCR reported excellent concordance (0.99). The sensitivity and specificity of MALDI-TOF MS for the diagnosis of opportunistic pathogenic yeasts of clinical samples were 94.6% and 99% respectively. MALDI-TOF MS is a simple, fast and reliable tool for pathogenic yeasts.
Assuntos
Humanos , Micoses , Leveduras , Candida/genética , Sensibilidade e Especificidade , Espectrometria de Massas por Ionização e Dessorção a Laser Assistida por MatrizRESUMO
Um estudo de metanálise avaliou a relação entre a espessura de toicinho e as variáveis de condição corporal de porcas gestantes e lactantes. A base de dados contemplou 14 artigos publicados de 2000 a 2006 em revistas indexadas. A metanálise foi realizada através de análises gráfica, de correlação e de variância. A correlação da espessura de toicinho (ET) com o peso vivo foi de 0,16 (P<0,01), com a massa protéica de 0,48 (P<0,01) e com a concentração de leptina de 0,88 (P<0,01). A correlação da variação da espessura de toicinho na lactação (ETl) com o peso vivo foi de -0,21 (P<0,01), com variação do peso vivo na lactação de 0,34 (P<0,01) e com variação da massa lipídica na lactação de 0,70 (P<0,01). A correlação entre a ET e o número de leitões nascidos vivos foi de 0,46 (P<0,01), e entre a ETl e o PV dos leitões aos sete dias foi de 0,95 (P<0,01). A ET foi influenciada pelo peso vivo e pela massa protéica na gestação, enquanto a ETl é influenciada pela variação do peso vivo e pela massa lipídica na lactação. As concentrações de leptina ao parto estão correlacionadas positivamente com a ET. A ET é influenciada pelo número total de leitões nascidos vivos e pelo peso vivo dos leitões ao nascimento, enquanto a ETl é influenciada pelo peso vivo dos leitões aos sete dias e pelo ganho de peso vivo da leitegada. Há relação significativa entre espessura de toicinho e variáveis de condição corporal de porcas gestantes e lactantes.
A meta-analysis was carried out to evaluate the association between backfat thickness and sow body condition in gestation and lactation. The database assembled 14 publications from 2000 to 2006. The meta-analysis was accomplished by graphical analysis, correlation, and analysis of variance. The correlation between backfat thickness (BT) and body weight was 0.16 (P<0.01), with protein mass was 0.48 (P<0.01) and leptin concentration was 0.88 (P<0.01). The correlation between the backfat variation during and in lactation (VBTl) and body weight was -0.21 (P<0.01), with body weight variation in lactation was 0.34 (P<0.01) and with fat mass variation in lactation was 0.70 (P<0.01). The correlation between BT and born alive litter size was 0.46 (P<0.01), between VBTl and piglets body weight at seven days of age was 0.95 (P<0.01). In the gestation, the BD was influenced by the body weight and protein mass. However, in lactation the VBTl was influenced by the body weight variation and fat mass. The leptin concentration at farrowing was positively correlated with backfat depth. The BT was influenced by born alive litter size and piglets birth weight. The VBTl was influenced by piglets weight at seven days old and litter weight gain. In conclusion, there is a significant relation between backfat thickness and body variables of the sows in gestation and lactation.