The involvement of amino acids in latex lipid synthesis in Euphorbia lathyris seedlings

The breakdown of triglycerides and proteins in the endosperm of Euphorbia lathyris was assayed in a 14 day germination period. Six days after germination, the average daily production was 2.7 μmol of amino acids. Arginine, glutamine, asparagine and glutamic acid accounted for 53% of the total amino acids. Excised cotyledons with 1 cm hypocotyls were used for amino acid uptake and their involvement in terpenoid synthesis was studied. Glutamine and aspartate were hardly involved in apolar lipid synthesis. Leucine, isoleucine, valine and threonine were mainly incorporated into the triterpenes in the laticifers. Alanine and serine were also involved in phytosterol synthesis in the adjacent tissue. In the 14 day germination period, ca3% of the daily yield of latex triterpenes may be synthesized from a variety of amino acids.     

Quantitative aspects of triacylglycerol metabolism and sterol synthesis from 14C-acetate in etiolated seedlings of Euphorbia lambii

Triacylglycerols occur in both the endosperm and embryo of Euphorbia lambii seeds. Upon germination, the amount of these neutral lipids in the endosperm decreased with 1.06 mg fatty acid day^-1. The embryo contained 1.4 mg fatty acids in the triacylglycerols and this value declined slowly to 0.4 mg seedling^-1 during the 8 day period of endosperm depletion. Radioactive acetate was rapidly taken up by the cotyledons of intact seedlings, translocated throughout the entire seedling, and up to 10.5% of the ¹⁴C proceeded to the sterols and latex triterpenols. Maximum uptake values of 1.4 μmol seedling^-1 day^-1 of acetate were measured. Acetate uptake and subsequent incorporation into sterols and triterpenols decreased substantially in the presence of increasing amounts of sucrose (up to 0.3 M). Traces of acetate did not effect [¹⁴C]-sucrose uptake and corresponding synthesis of [¹⁴C]-sterols and triterpenols, but increased concentrations of acetate (0.05 M and up) reduced both uptake of sucrose and its conversion into unsaponifiable lipids.
The uptake capacity of the cotyledons for [¹⁴C]-glycerol exceeded the daily production in the endosperm, but only a small amount of label proceeded to the sterols and triterpenols. [¹⁴C]-Triacylglycerols were never detected in the seedling, regardless of the labeled substrate used. Although acetate is an efficient precursor in triterpenol and sterol synthesis, the uptake capacity of the cotyledons for this metabolite is too small in relation to the daily production of water soluble substrates in the endosperm. If acetate is released by the endosperm, only a marginal contribution towards triterpenol and sterol synthesis in the seedling is to be anticipated from this substrate.     

Organic acids and cellular changes in the endosperm of Euphorbia lambii seedlings

Seedling of Euphorbia lambii Svent. were grown in the dark, and the levels of organic acids in the endosperm were monitored during the 6–7 day period in which all the reserves were depleted. Glycolate, glyoxylate, succinate, fumarate and 2-oxoglutarate occurred in traces only, the citrate concentration remained rather constant (0.4 μmol endosperm^?1), malate varied from 0.2 to 0.4 μmol endosperm^?1, but malonate appeared to be the major organic acid in the endosperm ranging from 0.75 to 1.25 μmol endosperm^?1. Radioactive malonate was easily taken up by the cotyledons of growing seedlings, and up to 11.2% of the label proceeded to the sterols, the triterpenes and triterpene esters in a 48 h incorporation period. No label from [¹⁴C]-malonate was built into the triacylglycerols in the seedling. Maximum uptake values of 0.6 μmol malonate seedling^?1 day^?1 were measured, and this value was not altered by a simultaneous uptake of sucrose. Conversely, the uptake of labeled sucrose and its subsequent conversion into sterols and (latex) triterpenes was not altered by a simultaneous uptake of low concentrations of malonate. Increased amounts (from 0.25 μmol malonate seedling^?1 and up) caused a 75–90% reduction of both uptake and conversion of sucrose into neutral lipids. To maintain a daily uptake of 4 μmol of sucrose by the cotyledons (required to maintain seedling growth) the simultaneous in vivo uptake of malonate from the endosperm was supposed not to exceed 0.2 μmol seedling^?1 day^?1. Thin sections of the endosperm revealed the morphology of the process of reserve depletion. The occurrence of vacuoles 2 days after germination, coincided with the increase in the malonate level. The protein bodies first disappeared completely from the outer layers, whereas the triacylglycerols gradually disappeared from the entire endosperm. About 80% of the endosperm cells contained a large vacuole until the stage of complete depletion, probably serving as the major site of malonate storage.     

Tapping-mode atomic force microscopy produces faithful high-resolution images of protein surfaces.

Compared to contact-mode atomic force microscopy (CMAFM), tapping-mode atomic force microscopy (TMAFM) has the advantage of allowing imaging surfaces of macromolecules, even when they are only weakly attached to the support. In this study, TMAFM is applied to two different regular protein layers whose structures are known to great detail, the purple membrane from Halobacterium salinarum and the hexagonally packed intermediate (HPI) layer from Deinococcus radiodurans, to assess the faithfulness of high-resolution TMAFM images. Topographs exhibited a lateral resolution between 1.1 and 1. 5 nm and a vertical resolution of approximately 0.1 nm. For all protein surfaces, TMAFM and CMAFM topographs were in excellent agreement. TMAFM was capable of imaging the fragile polypeptide loop connecting the transmembrane alpha-helices E and F of bacteriorhodopsin in its native extended conformation. The standard deviation (SD) of averages calculated from TMAFM topographs exhibited an enhanced minimum (between 0.1 and 0.9 nm) that can be assigned to the higher noise of the raw data. However, the SD difference, indicating the flexibility of protein subunits, exhibited an excellent agreement between the two imaging modes. This demonstrates that the recently invented imaging-mode TMAFM has the ability to faithfully record high-resolution images and has sufficient sensitivity to contour individual peptide loops without detectable deformations.     

Mobilisation of reserves and the earliest synthesis of sterols and latex triterpenes during germination and early seedling growth of Euphorbia lathyris

Seedlings of Euphorbia lathyris L. were grown in the dark at 25°C. Levels of amino acids, sugars and soluble phosphate in the endosperm increased upon germination after 4 days of imbibition, while the amounts of mineral reserves Mg²⁺ and K⁺ started decreasing. Ca²⁺ was not translocated from the endosperm to the seedling. Maximum values for amino acids were found on day 7, and the highest amounts of sugars were present on day 10. The endosperm was completely depleted by day 12.
Before germination (days 1–3) a low level of sterol synthesis in the embryo was detected with labeled sucrose and serine and to a lesser extent with labeled pyruvate. The label of [2-¹⁴C]-mevalonate proceeded exclusively to squalene. Laticifers started the synthesis of their triterpenes upon germination (day 4), using sucrose as a main substrate. A concurrent increase of sterol synthesis outside the laticifers was traced with labeled serine. Radioactive triterpenes, 4 α-methylsterols and sterols were detected in growing seedlings after [¹⁴C]-mevalonate uptake, but most of its label accumulated in squalene. The use of labeled mevalonate in sterol synthesis in growing seedlings is discussed.     

Direct visualization of phosphorylase-phosphorylase kinase complexes by scanning tunneling and atomic force microscopy.

In skeletal muscle the activation of phosphorylase b is catalyzed by phosphorylase kinase. Both enzymes occur in vivo as part of a multienzyme complex. The two enzymes have been imaged by atomic force microscopy and the results compared to those previously found by scanning tunneling microscopy. Scanning tunneling microscopy and atomic force microscopy have been used to view complexes between the activating enzyme phosphorylase kinase and its substrate phosphorylase b. Changes in the size and shape of phosphorylase kinase were observed when it bound phosphorylase b.