Porous graphitic carbon chromatography-tandem mass spectrometry for the study of isoprostanes in human cerebrospinal fluid

F2-isoprostanes are produced by the non-enzymatic peroxidation of arachidonic acid in membrane phospholipids. This paper describes a new method for the determination of all four classes of F2-isoprostanes in human cerebrospinal fluid (CSF) involving separation on a 1 mm x 150 mm porous graphitic carbon (PGC) column and detection by triple quadrupole mass spectrometry in negative-ion electrospray mode. The sample pre-treatment consisted of an ultrafiltration step, following which 300 microl of CSF sample could be injected directly onto a 1 mm x 10 mm PGC guard column functioning as a trap for the analytes. The loading solvent was Milli-Q water at 125 microl/min. After 3 min, the sample was switched into the separation column. The F2-isoprostanes were separated in 20 min using a linear solvent gradient comprising water, methanol, acetonitrile and ammonium hydroxide at a pH of 9.5 and a flow of 50 microl/min The limit of detection (calculated as 3S/N) was approximately 40 pM (14 pg/ml). The assay was linear within the examined range (18-450 pg/ml), using CSF spiked with iPF2alpha-III standard (r(2)>0.995). Repeatability data were calculated for CSF spiked to 90 pg/ml and the relative standard deviation (RSD) obtained was 3% (n=6).     

一种有效的花瓣总RNA的提取方法

利用CTAB法以富含花青素类物质的紫蓝色花瓣为材料提取总RNA,经紫外光谱分析A260/A280比值为1.9~2.0,A260/A230比值约为2.0;电泳检测到了28S、18S和5S rRNA清晰的条带;通过RT-PCR扩增出了目的基因的cDNA片段,说明分离的总RNA能去除色素干扰,纯度和反转录活性较高符合RNA相关实验的要求,是一种经济、有效的花瓣总RNA的提取方法。     

A comparison of venation pattern development in wild type and a homeotic sepaloid petal mutant of Clarkia tembloriensis (Onagraceae)

Vascular system development in sepals, petals, and sepaloid petals was compared in wild-type and crinkled petal mutant plants of Clarkia tembloriensis. Patterns of vascularization in cleared whole mounts were visualized and traced under both brightfield and polarizing illumination. Wild-type sepals exhibited a basipetal pattern of maturation, with tracheary elements maturing relatively rapidly. Mature sepals had three primary veins with numerous secondary veins. In contrast, wild-type petals exhibited an acropetal pattern of maturation, with tracheary elements maturing relatively slowly. The mature petals had only one primary vein with numerous secondary veins. Sepaloid (crinkled) petals combined characteristics of both wild-type sepals and wild-type petals. They exhibited a basipetal pattern of development and a relatively rapid maturation of the tracheary elements characteristic of wild-type sepals. Venation architecture in crinkled petal mutants showed a single primary vein with numerous secondary veins, similar to wild-type petals. The crinkled petal mutant fits the definition of a homeotic mutant in that the petal has assumed characteristics of the sepal. However, homeotic transformation from petal to sepal is incomplete since the crinkled petal still retains many of the characteristics of wild-type petals.     

Flower development and vasculature in Xyris grandis (Xyridaceae,Poales); a case study for examining petal diversity in monocot flowers with a double perianth

Floral morphology, anatomy and development are examined in Xyris grandis (Xyridaceae: Poales), with an emphasis on petal and sepal organogenesis and vasculature. Xyris is one of relatively few monocots in which the perianth is differentiated into two distinct whorls (here termed a double perianth). Xyris also possesses highly unusual perianth vasculature, with each petal being supplied by three veins and each sepal by a single vein, compared with the opposite condition in most other angiosperms with a double perianth. However, perianth development in X. grandis shows a pattern that is typical for monocots, with petals not markedly delayed in development. Xyris grandis is also remarkable for its petal aestivation, with each petal surrounding a stamen and two branches of adjacent staminodes, a type that is not reported for other Xyridaceae and may contribute to secondary pollen presentation. The results are discussed in the context of the diversity of a double perianth in monocots, compared with eudicots. Based on current data, our preferred hypothesis is that meristic differences are at least partly responsible for the apparently widespread occurrence of three‐traced petals in monocots. © 2012 The Linnean Society of London, Botanical Journal of the Linnean Society, 2012, 170 , 93–111.     

Elaborate petals in Australian Spermacoce (Rubiaceae) species: morphology, ontogeny and function

BACKGROUND AND AIMS: Australian Spermacoce species display various types of elaborate petals. Their precise morphology, ontogenetic origin, and function are hitherto unknown. The aim of the present paper is to unravel the development and nature of the diverse types of elaborate petals in Spermacoce through a floral ontogenetic study. METHODS: The floral ontogeny of six species characterized by different types of corolla appendages was studied by scanning electron microscopy and light microscopy. In order to elucidate the possible functions of the elaborate petals, field observations were conducted as well. KEY RESULTS: Scanning electronmicrographs show that full-grown petals of Spermacoce lignosa, S. phaeosperma and S. redacta bear appendages on their ventral side. Despite their different appearance at anthesis, the appendages develop very similarly in all three species. They are initiated at the same developmental stage and are first visible as two arcs of primordia converging from the upper margins of the petal towards its midvein and downwards. In S. brevidens, S. caudata and S. erectiloba, the full-grown petals have two long, concave protuberances, which develop from the tissue at both sides of the petal's mid-vein. In these three species, initiation of appendages on the ventral side of the petals is also observed, but they are hardly visible on the mature petals. The two types of elaborate petals tightly enclose the anthers, both in bud and during most of the flowering period. CONCLUSIONS: Among Australian Spermacoce species, two types of elaborate petals can be distinguished. The former hypothesis that the two types of elaborate petals are essentially homologous is here rejected. Field investigations point out that the elaborate petals might play a role in the pollination biology of the species.     

Floral morphogenesis in Sinofranchetia (Lardizabalaceae) and its systematic significance

The floral organs of Sinofranchetia chinensis Hemsl. (Lardizabalaceae) are all spiral in initiation. Stamen and petal (nectar‐leaf) primordia initiate independently and are different in shape. The petals and three stamens in the first whorl are retarded in the early developmental stages. The carpel primordia are conduplicate; the stigma is formed around the upper part of the ventral slit and the style is not differentiated. The functionally unisexual flowers are bisexual in organization in the early developmental stages. The development of the flowers on the inflorescence is spiral and centripetal. Some floral characteristics of Sinofranchetia appear to be plesiomorphic in Lardizabalaceae. © 2009 The Linnean Society of London, Botanical Journal of the Linnean Society, 2009, 160 , 82–92.     

Determination of isoprostanes in urine samples from Alzheimer patients using porous graphitic carbon liquid chromatography-tandem mass spectrometry

F2-isoprostanes (F2-iPs) comprise four classes of isomers produced non-enzymatically by free radical attack on arachidonic acid, a component of the cell membrane. This paper describes a new method for the quantification of F2-isoprostanes in urine samples from thoroughly diagnosed Alzheimer's disease (AD) patients. The sample pretreatment consisted of liquid extraction of 900 microl urine with diethyl ether, its subsequent evaporation, and finally, reconstitution in 50 microl water. Of this, 20 microl was injected into a HPLC system with a 15 mm x 1 mm porous graphitic carbon column coupled to a triple quadrupole mass spectrometer running in negative electrospray ionization mode. The F2-isoprostanes were separated in 15 min using a linear solvent gradient comprising water, methanol, acetonitrile and ammonium hydroxide at a pH of 9.5. The average recovery obtained was approximately 75%. The limit of detection (3S/N) was calculated for iPF2alpha-III to be 0.7 pg injected on column, corresponding to 0.1 nM. The average level of iPF2alpha was 241 +/- 163 pg/mg creatinine in the urine samples from AD patients (average +/- standard deviation). The corresponding control values were 216 +/- 101 pg/mg creatinine, i.e. no statistically significant difference was noticed. No correlation pattern specific to Alzheimer's disease was revealed by principal component analysis of the isoprostane peaks obtained either. The results from this study support earlier findings that levels of peripheral isoprostanes are not increased in patients with Alzheimer's disease.