Functional and DNA sequence divergence of the CYP71 gene family in higher plants.

During ripening of avocado (Persea americana), the CYP71A1 mRNA and protein accumulate to relatively high levels. Although the CYP71A1 gene was the first plant P450 to be cloned and sequenced, the functional role of this P450 remains obscure. Substrate studies have shown that CYP71A1 will metabolize various monoterpenes (nerol and geraniol), although these have not been detected in ripening fruit. Using DNA from a conserved domain of the CYP71A1 gene, we have explored the scope of the CYP71 (or related) gene family in avocado using low stringency DNA hybridization. This analysis suggests that there are approximately 10-12 genes in the CYP71 family. An alternative approach using PCR gave essentially identical results.

Plant cytochrome P450.

The present status of plant cytochrome P450 research is reviewed. A comparison of the properties of this group of cytochrome proteins with those of other microsomal b-type haem proteins is made. The range of reactions catalysed by P450s is discussed as well as recent progress in improving purification and reconstitution. Molecular cloning approaches that have overcome the earlier block to accessing this gene superfamily are discussed and future prospects highlighted. Expression of the gene family is discussed in relation to regulation in response to environmental and developmental cues and tissue and subcellular localization. The biotechnological importance of this gene family is stressed.

Expression of a Ripening-Related Avocado (Persea americana) Cytochrome P450 in Yeast.

One of the mRNAs that accumulates during the ripening of avocado (Persea americana Mill. cv Hass) has been previously identified as a cytochrome P450 (P450) monooxygenase and the corresponding gene designated CYP71A1. In this report we demonstrate that during ripening the accumulation of antigenically detected CYP71A1 gene product (CYP71A1) correlates with increases in total P450 and two P450-dependent enzyme activities: para-chloro-N-methylaniline demethylase, and trans-cinnamic acid hydroxylase (tCAH). To determine whether both of these activities are derived from CYP71A1, we have expressed this protein in yeast (Saccharomyces cerevisiae) using a galactose-inducible yeast promoter. Following induction, the microsomal fraction of transformed yeast cells undergoes a large increase in P450 level, attributable almost exclusively to the plant CYP71A1 protein. These membranes exhibit NADPH-dependent para-chloro-N-methylaniline demethylase activity at a rate comparable to that in avocado microsomes but have no detectable tCAH. These results demonstrate both that the CYP71A1 protein is not a tCAH and that a plant P450 is fully functional upon heterologous expression in yeast. These findings also indicate that the heterologous P450 protein can interact with the yeast NADPH:P450 reductase to produce a functional complex.

Avocado fruit protoplasts: a cellular model system for ripening studies.

Mesocarp protoplasts were isolated from mature avocado fruits (Persea americana cv. Hass) at varying stages of propylene-induced ripening. Qualitative changes in the pattern of radiolabel incorporation into polypeptides were observed in cells derived from fruit at the different stages. Many of these differences correlate with those observed during radiolabeling of polypeptides from fresh tissue slices prepared from unripe and ripe fruit. Protoplasts isolated from fruit treated with propylene for one day or more were shown to synthesize cellulase (endo-ß-1,4-glucanase) antigen, similar to the intact propylene-treated fruit. These results suggest that the isolated protoplasts retain at least some biochemical characteristics of the parent tissue. The cells may also be used in transient gene expression assays. Protoplasts isolated from preclimacteric and climacteric fruit were equally competent in expressing a chimeric test gene, composed of the CaMV 35S RNA promoter fused to the bacterial chloramphenicol acetyltransferase gene, which was introduced by electroporation.

Sequence analysis of ripening-related cytochrome P-450 cDNAs from avocado fruit.

The ripening of avocado fruit is associated with the expression of a number of mRNAs concomitant with overt changes in texture and flavor. Two overlapping cDNAs for a mRNA that accumulates during ripening were identified. Sequence analysis of these two cDNAs revealed a polypeptide of 471 amino acids with characteristics of a typical P-450: an N-terminal hydrophobic membrane anchor, a conserved heme-binding domain in the C-terminal region, and patches of similarity to various P-450 family members. Further evidence that this polypeptide represents a cytochrome P-450 oxidase comes from the recent isolation and characterization of a cytochrome P-450 from ripe avocado mesocarp [O'Keefe, D. P. & Leto, K. J. (1989) Plant Physiol. 89, 1141-1149]. The N terminus of the predicted polypeptide in the cDNAs is identical to the N terminus of the purified avocado P-450. Gel blot analysis of RNA from fruit at various stages of ripening showed the accumulation of an 1800-nucleotide P-450 mRNA that hybridized to the P-450 cDNA. The P-450 protein predicted by the avocado cDNA sequence shares less than 40% positional identity with any known P-450 gene family. We propose therefore that it be placed in a separate family, P450LXXI, and that the corresponding gene from avocado be named cyp71A1.

In vitro rat myocyte cardiotoxicity model for antitumor antibiotics using adenosine triphosphate/protein ratios.

Cumulative cardiotoxicity consistently limits the use of antitumor anthracyclines such as doxorubicin (DOX). Several in vivo and in vitro model systems have been developed for screening cardiotoxic agents. Problems with these models include excessive time and nonquantitative toxicity end points. We describe an in vitro system for culturing cardiac myocytes which overcomes these problems. Optimal myocyte cultures were obtained using serial 0.2% crude trypsin digestions of hearts from 1-2-day-old rats. Three-day-old myocyte cultures were treated with DOX for 6 h at concentrations of 0.1 to 10 micrograms/ml (0.18 to 18 microM). Electron microscopy performed on control and DOX-treated cultures showed characteristic histopathological signs of anthracycline damage. These changes included mitochondrial swelling, nuclear pleomorphism, chromatin clumping, and a diffuse loss of membrane integrity. Intracellular ATP, quantitated by the luciferase bioluminescence method, was shown to provide a simple and consistent quantitative biochemical marker of myocyte viability over the range of DOX concentrations used. The results showed both time- and dose-dependent decrements in ATP/protein ratios 72 h following exposure to DOX at concentrations greater than 0.1 microgram/ml. Leakage of lactate dehydrogenase activity, trypan blue uptake, and myocyte beating rates were variable and not as sensitive as ATP levels for evaluation of myocyte viability. Other cytotoxic agents which are not known to be cardiotoxic (dactinomycin, 1-beta-D-arabinofuranosylcytosine, fluorouracil, melphalan, and vincristine), required extremely high concentrations to produce myocyte damage in vitro. Tests with anthracycline analogues also demonstrated the ability of the assay to rank-order cardiotoxic agents on a weight basis: idarubicin greater than DOX greater than daunomycin greater than aclarubicin. When the in vitro drug concentrations required to lower ATP/protein ratios to 50% of controls were related to clinically achievable concentration x time products, DOX and daunomycin proved to be the most cardiotoxic in this series. These results suggest that comparative cardiotoxic screening studies may be performed in vitro using ATP levels in beating neonatal myocytes.